Scale Up PDF

JOURNAL OF BIOSCIENCE AND BIOENGINEERING
Vol. 97, No. 6, 347364. 2004
Scale-Up Methodologies for Escherichia coli and

Yeast Fermentation Processes
BETH HELENE JUNKER1
Merck Research Laboratories, Bldg. 810-127, PO Box 2000, Rahway, NJ 07065, USA1
Received 22 August 2003/Accepted 15 March 2004
Scale-up techniques from the literature have been compiled and reviewed for applicability to
Escherichia coli and yeast processes. The consistency of design and operating parameters for the
pilot scale vessels in an existing fermentation pilot plant, ranging in nominal volume from 100 l to
19,000 l, was established and compared favorably with approaches found in the literature. Differ-
ences were noted as a function of parameters such as fermentor scale, vessel geometry, agitator
type/size and ungassed/gassed power input. Further analysis was conducted using actual fermen-
tation data for historical and recent development processes collected over a 10-year-period, focus-
sing on operating conditions at peak culture oxygen uptake rates. Scale-up estimates were per-
formed based on geometric similarity, agitator tip speed, gassed power per unit volume and mix-
ing time. Generally, scale-up calculations from the 280 l scale were most similar to the parameters
of installed equipment. Scale-up from the 30 l laboratory scale typically underpredicted parame-
ters with scale-up from the 280 l scale being most appropriate. The 19,000 l fermentor installation
was notably different in geometric similarity from the 280 l1900 l scales since its design was
meant to accommodate a wide range of operating volumes. Analysis of historical and recent proc-
essing performance was conducted for single cell bacterial or yeast fermentations which chal-
lenged peak operating conditions of the fermentors. Identification of key issues associated with
scale-up for these specific pilot plant vessels was believed to be critical to efficient process devel-
opment, clinical material production, and expected process transfer to a manufacturing facility.
[Key words: scale-up, Escherichia coli, yeast, pilot plant, fermentor]
General concerns for recombinant DNA scale-up have well. Additionally, the role of scale-down studies can be sig-
been addressed by Van Brunt (1). Although the three main nificant in identifying and evaluating problems at the large
scales for bioprocess development are laboratory, pilot plant scale (811).
and production (2), Votruba and Sobotka have added the Biological factors affected by scale include the number of
shake-flask scale to this list (3). The scale-up ratio is typi- generations associated with the inoculum development and
cally about 1 : 10 for biotechnological processes up to production phases, mutation probability, contamination vul-
100,000 l (3), but lower ratios of about 1 : 5 often have been nerability, pellet formation and selection pressure (8, 12).
used for increased comfort levels (i.e., decreased risk of Chemical factors affected by scale include (i) pH control
unexpected performance on scale-up). Production scale for agents (i.e., type and concentration of acid and/or base), me-
many recombinant DNA products is likely to be about dium quality (i.e., purity of components) and water quality
10,000 l which is more traditionally pilot scale for other (8); (ii) carbohydrate (e.g., oil), nitrogen (e.g., ammonia),
types of products (4). The exact methodology used for scale- phosphorus and product concentrations (6); (iii) redox po-
up is largely dependent on process conditions and whether tential and foam formation due to surface tension changes
preliminary data exist to show that the procedure chosen is (3). Physical factors affected by scale include tank configu-
applicable (5). ration, aeration, agitation, back-pressure (and hydrostatic
Some authors maintain that the total environment (Young pressure), medium sterilization, temperature control/heat
[6] coined this term to encompass all the chemical and transfer and removal, and mixing (3, 8, 12).
physical variables relating to the fermentor broth) of the cell There is a comprehensive paper outlining general ap-
needs to be considered (6). A complete catalog of factors proaches to scale-up (13) and it includes comments from
affected by scale is detailed extensively by Reisman (7) several other authors on the implications of general trends
with key items being emphasized by other authors (16) as in scale-up. Unless specifically maintained constant with
scale-up to the larger fermentor, dissolved carbon dioxide
e-mail: Beth_Junker@Merck.com (dCO2) is higher in the larger vessel than the smaller vessel
phone: +1-732-594-7010 fax: +1-732-594-7698 due to the added head pressure, shear force variation is
347
348 JUNKER J. BIOSCI. BIOENG.,
higher, and bulk mixing is less efficient due to longer circu- gen transfer. For the scale-up of toyocamycin production by
lation times and larger stagnant regions (8). In addition, for a shear-sensitive mutant of Streptomyces chrestomyceticus,
the larger vessel, the liquid height to tank diameter ratio can neither the constant Pg/VL method nor the constant OTR
be greater, gas moves upwards with more limited backmix- method could be used, and thus scale-up was done at the
ing, vertical dissolved oxygen (DO) gradients exist if bulk lowest possible tip speed for the geometrically similar larger
mixing is slower than mass transfer rates, and radial DO vessel (20). Mixing and circulation times were found to be
gradients emerge since the shear rate declines rapidly with more important than using constant oxygen uptake rate
distance from the impeller (14). Other trends in scale-up in- (OUR) for the scale-up of a 2,3-butanediol fermentation by
clude decreased heat transfer surface to volume ratio, de- Enterobacter aerogenes under microaerobic conditions in
creased quality of mixing, generally higher superficial air which homogeneity was important (21). Although, in gen-
velocity, and lower average shear force although peak shear eral, the scale-up based on dCO2 would be even more feasi-
forces are higher (14, 15). Furthermore, if cheaper medium ble as more reliable dCO2 sensors become available (16),
components have been selected with variable composition the specific carbon dioxide evolution rate was currently still
for different bulk lots, a previously unnoticed auxotrophic felt to be useful for scale-up of secondary metabolite cul-
growth pattern may appear (15), but this occurrence is mini- tures (22).
mized by the use of defined medium. The purpose of this paper is to briefly describe and evalu-
There are several published descriptions of scale-up stud- ate various scale-up methods and approaches which can be
ies and a few interesting examples are noteworthy. Oxygen applied to example E. coli and yeast processes. The first
transfer often can be most important upon scale-up due to step involved cataloging characteristic measurements for ex-
its low solubility in medium (16). Key to scale-up using isting laboratory (30 l scale) and pilot plant (100 l19,000 l
constant oxygen transfer rate (OTR) is the ability to mea- scale) fermentors (Tables 1 and 2). Next, relevant parame-
sure or estimate the volumetric mass transfer coefficient, ters were calculated and compared as a function of scale
KLa, and the gassed power per unit liquid volume, Pg/VL. based on geometry, power input per unit volume, gas flow
Published correlations can generate significant errors as in rate and mixing time (Tables 35). Various scale-up scenar-
the example of KLa factors for a commercial-scale penicillin ios were explored based on maintaining geometric similar-
fermentation (17). The scale-up of bialaphos production by ity (Table 6), constant impeller speed (Table 7), and con-
Streptomyces hygroscopicus based on KLa and Pg/VL was stant power input per unit liquid volume (Tables 8 and 9). A
not successful due to the large DO concentration gradients comparison was also completed based on medium heat
in the fermentor (18). In this example, the culture was not stress during sterilization (Table 10). A listing of historical
sensitive to impeller tip speed changes upon scale-up. Scale- and recent achievable processing conditions was developed
up was successful when the target DO in the laboratory fer- (Tables 11 and 12), and the relationship of OUR to KLa and
mentor was used to control the large scale fermentor DO us- Pg/VL to KLa was quantified for various processes (Table
ing a probe located at the bottom of the large scale fermen- 13). For consistency, all volumes quoted in this text are
tor. Similarly, scale-up deteriorated production syndrome nominal vessel volumes (rather than total or working vol-
(SUDS) was observed during the scale-up of milbemycin umes) unless otherwise stated. Units were selected to mini-
production by S. hygroscopicus when agitation rate was used mize rounding errors where possible.
to control DO as was done at the small scale (19). SUDS
syndrome included culture morphological changes which
I. SCALE-UP METHODS AND APPROACHES
affected packed cell volume and viscosity, carbon source
uptake changes, and decreased productivity. An alternative Several scale-up methods are described below, and se-
DO control strategy using aeration rate, back-pressure, tem- lected scale-up approaches were evaluated using two scales
perature, in addition to agitation rate, was developed to as a basis: the 280 l pilot scale which is a common first step
maintain laboratory yields upon scale-up. pilot plant fermentor scale and the 30 l laboratory scale
Additional examples focus on parameters other than oxy- which is common to use for pre-pilot plant (laboratory) stud-
TABLE 1. Characteristics of laboratory and pilot scale vessels

Vessel
Vessel
Working Installed Max. Vessel total height Max.
Scale width,
tank volume, motor power, agitator speed, tangent/tangent, (with top and air flow rate,
(nominal volume) OD,
VL (l) Po (hp) Nmax (rev/min) HTT (m) bottom dish), Qmax (l/min)
DT (m)
HT (m)
30 l 20 1 875 0.66 0.742 0.31 30
100 l 75 3 400 0.785 0.96 0.41 (ID) 120
280 l 180 7.5 460 1.12 1.34 0.56 300
800 l 600 7.5 330 1.63 2.08 0.81 600
1000 l 750 10 300 1.52 1.88 0.86 (ID) 1200
1200 l 900 15 282 1.83 2.185 0.92 1200
1900 l 1500 15 230 2.13 2.57 1.07 1500
19000 l 15000 60 155 5.87 6.58 1.98 15000
The 280 l scale fermentor was originally designed with a 3 hp motor which was enlarged to 7.5 hp for replacement convenience. OD, Outer di-
ameter; ID, inner diameter.
VOL. 97, 2004 SCALE-UP METHODOLOGIES FOR FERMENTATION PROCESSES 349
TABLE 2. Characteristics of laboratory and pilot-plant scale impellers

Scale Impeller type Impeller diameter, Impeller tip speed, Number of
(nominal volume) (upper/lower) DI (m) pNmaxDI (m/s) impellers, NI
30 l Rushton 0.102 4.7 4
100 l Hydrofoil 0.184 3.8 2
A315
280 l Rushton 0.205 4.9 2
Hydrofoil 0.28 6.7 3
Maxflo T
800 l Rushton 0.305 5.4 2
Maxflo T
A315
Smith Top, 0.343 Top, 6.1 2
CD-6 Btm, 0.356 Btm, 6.3
Hydrofoil/Smith Top, 0.406 Top, 7.2 2
Maxflo T/CD-6 Btm, 0.394 Btm, 7.0
HE-3/Smith Top, 0.533 Top, 9.4 2
HE-3/CD-6 Btm, 0.394 Btm, 7.0
1000 l Rushton 0.305 4.8 2
A315
1200 l Hydrofoil 0.46 6.8 2
A315
1900 l Rushton 0.42 5.1 3
Maxflo T
19000 l Rushton 0.685 5.6 4
Maxflo T
Hydrofoil Top/Mid, 0.94 7.6 3
A315 (Btm, 8.4) (Btm, 8.4)
Impeller data for top/bottom impellers. Units of length selected to minimize rounding errors. Top, Top impeller; Mid, middle impeller; Btm, bot-
tom impeller.
TABLE 3. Geometric comparisons for laboratory and pilot scale fermentors

Scale HT/DT DT/(VL)1/3 at VL (l), Re106
DI/DT VL/VT
(nominal volume) (HTT/DT) geometric similarity (water)
30 l 2.4 0.33 (R) 1.14 at 20 0.48 (R) 0.57
(2.1)
100 l 2.4 0.45 (A) 0.97 at 75 0.71 (A) 0.75
(1.9)
280 l 2.4 0.36 (R) 0.99 at 180 1.0 (R) 0.60
(2.0) 0.5 (M) 1.9 (M)
800 l 2.6 0.38 (R) 0.96 at 600 1.6 (R) 0.704
(2.0) 0.5 (M) 2.9 (M)
0.5 (A) 2.9 (A)
1000 l 2.1 0.35 (R) 0.95 at 750 1.5 (R) 0.75
(1.7) 0.43 (A) 2.2 (A)
1200 l 2.4 0.5 (A) 0.95 at 900 3.1 (A) 0.75
(2.0)
1900 l 2.4 0.39 (R) 0.935 at 1500 2.1 (R) 0.79
(2.0) 0.5 (M) 0.96 at 1400 3.4 (M)
19000 l 3.3 0.346 (R) 0.80 at 15000 3.8 (R) 0.79
(2.9) 0.462 (M) 0.95 at 9000 6.8 (M)
0.47 (A) 7.2 (A)
(Btm, 0.56) (Btm, 8.8)
VT is total tank capacity not nominal volume. R, Rushton; M, Maxflo T; A, A315; Btm, bottom impeller.
ies. Details of some of these vessels and their impellers have Geometric similarity of reactor geometry [DT/VT)1/3 or
been discussed elsewhere (2325). Figure 1 shows a typical (DT/VL)1/3] Geometric similarity is expressed as follows:
fermentor diagram with key locations identified.
DT2/DT1 = (VT2/VT1)1/3 (1)
where DTi is the tank diameter and VTi is the total tank vol- Fermentors with a standard geometry are beneficial since
ume of vessel, i. Alternatively, the liquid volume, VLi, might several published scale-up correlations assume geometry to
be used. It assumes reasonably constant impeller geometry be constant (8). However, lab fermentors may have substan-
(i.e., impeller diameter, DI, and number of impellers, NI) as tially lower HT/DT ratios of 1:1 compared to 3:1 for pilot
specified below. Based on target working/total volumes ob- scale fermentors, so laboratory scale data may be deceiving
tained from geometric similarity (Table 6), the desired work- (8). Larger pilot scale and production fermentors can be de-
ing volume in the fermentor may be altered during experi- signed for variable working volumes to accommodate the
mentation. larger range of batch sizes expected in a multi-use facility.
Experiments to obtain data for several empirical correla- Table 6 shows the scale-up parameters of expected total
tions utilized geometrically similar vessels. Although geo- and working volumes calculated based on geometrical simi-
metric similarity is a pre-requisite for applying established larity. For the 280 l scale-up basis, the calculated numbers
scale-up relationships, it is rarely achievable in practice (26, differed dramatically from installed equipment for the 30 l
27). Subsequently, a range of acceptance of equivalency and 19,000 l scales, but were reasonably close (within 2
was proposed (26) to include the following: (i) DI/DT = 0.3 17%) between the 100 l and 1900 l scales. Although the
0.45, where DI/DT is the ratio of the impeller to tank diame- 19,000 l expected values were lower by 3047%, the 30 l
ters; (ii) HL/DT is less than or equal to 2 (no range was value was higher by 4655%. For the 30 l scale-up basis, all
given), where HL is the height of the liquid in the vessel; and the calculated numbers were substantially lower than the in-
(iii) either two or three impellers. As shown in Table 3, stalled values by 1945% between the 100 l and 1900 l
DI/DT values ranged from 0.330.5 for all vessels in this fa- scales and 5265% for the 19,000 l scale. Reasons for these
cility. Specifically, the range was 0.330.39 for vessels with differences were evident by comparing values of the geo-
Rushton radial flow impellers (Lightnin, Avon, NY, USA), metric similarity parameter, (DT/VL)1/3, listed in Table 3. Val-
0.4620.5 for vessels with Maxflo T axial flow impellers ues for the 100 l to 1900 l scale ranged from 0.9350.99
(Chemineer, Dayton, OH, USA), and 0.430.56 for vessels (average of 0.958 0.019); values for the 30 l and 19,000 l
with A315 axial flow impellers (Lightnin). In the case of the
vessels studied, HT/DT ratios ranged from 2.13.3 where HT
is the total tank height. The range of the tangent-to-tangent
tank height to tank diameter ratio, HTT/DT (which was felt to
be more useful than HL/DT to compare since fermentor
working volumes may be variable), was 1.72.9, with the
value of 2.9 for the 19,000 l fermentor being well above the
remainder which ranged from 1.72.1. All vessels had two
or three impellers except for two of the three 19,000 l ves-
sels (those with Rushton and Maxflo T impellers) which had
four impellers.
FIG. 2. Decline of installed, ungassed and gassed power draw per

unit working volume as a function of scale for fermentors under study
at operating conditions listed in Table 1 and for impeller geometries
listed in Table 2. For all scales, 1.7< HTT/DT <2.9 and 1.0<Qmax/VL <1.67.
(a) For Rushton (R) geometry, 0.33< DI/DT <0.39, 4.7<ITS <5.6. (b)
For Maxflo T (M) hydrofoil geometry, 0.462<DI/DT <0.5, 6.4<ITS<7.4.
FIG. 1. Schematic of fermentor showing nomenclature. For A315 (A) axial flow geometry, 0.43< DI/DT <0.56, 5.8<ITS <7.6.
TABLE 4. Mixing time, power input and gas flow comparisons for laboratory and pilot scale fermentors
Pg/VL at Qmax Superficial
Mixing time, Po/VL Qmax/VL Gas flow
Scale Design and Nmax gas velocity,
Tmix from (observed (vvm at number,
(nominal Po/VL (observed Vs =
Eq. 10h in water) working NA =
volume) (hp/1000 l) in water) 4Qmax/(pDT2),
(s) (hp/1000 l at rpm) VL min1) Qmax/NmaxDI3
(hp/1000 l at lpm) (cm/s)
30 l 3.4 50.0 NI NI 1.5 0.66 0.032 (R)
100 l 13.4 40.0 NI NI 1.6 1.5 0.050 (A)
280 l 20.1 41.7 23.9 at 450 (R) 18.8 at 300 (R) 1.67 2.0 0.078 (R)
18.9 at 450 (M) 16.7 at 300 (M) 0.030 (M)
800 l 29.2 12.5 15.0 at 335 10 at 600 (R) 1.0 2.0 0.063 (R)
12.5 at 300 (R)
16.3 at 335* 8.8 at 600 (M) 0.027 (M)
12.1 at 300 (M)
11.2 at 335 7.8 at 600 (A) 0.027 (A)
8.7 at 300 (A)
1000 l 30.9 13.3 7.7 at 300 (R) 4.3 at 1200 (R) 1.6 3.4 0.140 (R)
5.1 at 300 (A) 4.9 at 600 0.079 (A)
3.5 at 1200 (A)
4.6 at 600
1200 l 32.3 16.7 10.1 at 282 (A) 6.8 at 1200 (A) 1.33 3.0 0.044 (A)
7.1 at 600
1900 l 36.2 10.0 13.9 at 225 (R) 6.8 at 1500 (R) 1.0 2.8 0.088 (R)
10.0 at 225 (M) 8.0 at 1500 (M) 0.043 (M)
19000 l 53.7 4.0 4.4 at 142 (R) 2.0 at 15000 (R) 1.0 8.1 0.300 (R)
4.4 at 150 (M) 4.1 at 15000 (M) 0.130 (M)
4.4 at 150 (A) 3.2 at 15000 (A) 0.120 (A)
Power measurements performed at 25C in water and at ambient pressure. Unaerated conditions not maintainable at top speed for certain fer-
mentors marked with an asterisk due to drive overheating. No power measurement devices installed at 30 l or 100 l scales. R, Rushton; M, Maxflo T;
A, A315. NI, Power measuring device not installed.
TABLE 5. Mass transfer comparisons for laboratory and pilot scale fermentors
Scale Measured (Po/VL)a (Vs)b (Pg/VL)a (Vs)b
Vs at Qmax Qmax/VL
(nominal Pg/Po at using Eq. 9a and 9b using Eq. 9a and 9b
(cm/s) (vvm, min1)
volume/designation) Qmax and Nmax and design Po and measured Pg
30 l 0.66 1.5 NA 31.1 NI
100 l 1.5 1.6 NA 15.5 NI
280 l 2.0 1.67 0.79 (R) 19.4 11.3 (R)
0.88 (M) 10.5 (M)
800 l 2.0 1.0 0.67 (R) 8.6 7.4 (R)
0.54 (M) 6.8 (M)
0.70 (A) 6.3 (A)
1000 l 3.4 1.6 0.55 (R) 12.8 6.0 (R)
0.69 (A) 5.3 (A)
1200 l 3.0 1.33 0.67 (A) 13.8 7.5 (A)
1900 l 2.8 1.0 0.49 (R) 9.3 7.2 (R)
0.80 (M) 8.0 (M)
19000 l 8.1 1.0 0.45 (R) 10.3 6.5 (M)
0.93 (M) 10.4 (M)
0.74 (A) 8.8 (A)
The 1000 l scale fermentor was typically run at 600 lpm rather than at 1200 lpm maximum air flow rate which was used to obtain calculated and
measured values. Equation 9a used for 30 l scale and Eq. 9b used for 100 l19,000 l scales. Power measurements performed at 25C in water and at
ambient pressure. No power measurement devices installed at 30 l or 100 l scales. R, Rushton; M, Maxflo T; A, A315. NI, Power measuring device
not installed. NA, Calculation not applicable.
scales were notably different (greater than 4.59.5 SD from peller speed and impeller diameter for vessel i (8). Table 2
the mean). Operation of the 19,000 l scale fermentor at a shows that typical installed impeller tip speeds ranged from
lower working volume brings its geometrical similarity 3.8 to 7.6 m/s with no clear trend observed with scale, but
closer to the average value of the smaller vessels. about a 2537% increase with the hydrofoil (A315 and
Constant impeller tip speed (ITS) or shear ITS is Maxflo T) impellers than the disk turbine (Rushton) im-
expressed as pellers for the same fermentor scale primarily due to their
larger diameters.
N2/N1 = DT1/DT2 = (VT1/VT2)1/3 (2)
Tip speed is used as a rule for scale-up when there is not a
which assumes that ITS = pNi DIi where Ni and DIi are the im- good understanding of the relationship between shear and
morphology for mycelial cultures. A rough rule of thumb is late the values in Table 7, this explains why the 30 l and
that cell damage can occur at tip speeds above 3.2 m/s, but 19,000 l values were substantially different than installed
the exact value is influenced by many factors such as broth values and why the values for the 30 l scale-up basis were
rheology (28). Calculated tip speeds usually are greater than not in agreement as well.
3 m/s for production fermentors (29) and ranged from 57 Constant ungassed or (more often) gassed power input
m/s from a survey of industrial fermentors (Einsele, A., per liquid volume (Po/VL or Pg/VL) Scale-up designs
Abstr. 5th Intern. Ferment. Symp., p. 69, 1976). A constant may also include the ungassed power input, Po, which is ex-
tip velocity in the range of 57 m/s was found to be used pressed as
for scale-up for antibiotic fermentations (Einsele, Abstr. 5th
Po = NP N 3DI5r (3)
Intern. Ferment. Symp., 1976). Although useful in branched
yeast, filamentous bacterial and fungal fermentations for where NP, the power number, is a proportionality factor
estimating the potential for hyphae breakage and thus alter- based on the impeller design (among other factors) and r is
ation of broth morphology, tip speed is less useful for single the broth density (8) which is typically considered to be
cell bacterial or yeast fermentations. slightly greater than water. The power number generally re-
If scale-up is conducted using constant tip speed (with mains constant with scale-up if the same impeller type is
geometric similarity), then often the value of Pg/VL is low- used.
ered which can adversely affect aeration efficiency. It is Constant ungassed power, (Po/VL)i, for vessel, i, is ex-
possible to recover from this deficiency using more impel- pressed as
lers in the larger vessel and in this manner it may be pos-
(Po/VL)2/(Po/VL)1 = (VL1/VL2)c or Po/VL = f1VLc (4)
sible to maintain both tip speed and Pg/VL constant (30). Tip
speed influences impeller shear which is proportional to where c was found to be -0.37 in practice based on a survey
product of impeller tip speed and impeller diameter, NDI2, of industrial plants of various scales and processes (Einsele,
for turbulent flow conditions (29). Abstr. 5th Intern. Ferment. Symp., 1976). A similar rela-
As shown in Table 7, for the 280 l scale-up basis, there tionship can be applied for gassed power inputs. General
was reasonable agreement (within 224%) between ex- values of Po/VL are 13 kW/m3 (1.34 hp/1000 l) for vessels
pected and actual total and working volumes for the 280 l up to 300 m3 (300,000 l) working volume (Einsele, Abstr.
1900 l scales, but expected values were substantially lower 5th Intern. Ferment. Symp., 1976), and a rule of thumb is
(5869%) at the 19,000 l scale and grossly higher (97 that Po/VL is 24 kW/m3 (2.75.4 hp/1000 l) at the produc-
355%) for the 30 l and 100 l scales. For the 30 l scale-up tion scale with no volume range given by Kossen and
basis, all estimated values were substantially lower (40 Oosterhuis (29).
85%) than installed values, except for the 100 l vessel which If scale-up is conducted using constant Po/VL with geo-
was substantially higher (131175%) due to its higher peak metric similarity, then circulation time, mixing time and im-
agitation rate. Since geometric similarity was used to calcu-
TABLE 7. Scale-up based on constant impeller speed
TABLE 6. Scale-up based on geometric similarity a. Base case 280 l (pilot scale)
a. Base case 280 l (pilot scale) Scale Total Total Working Working
Scale Total Total Working Working (nominal volume, volume, volume, volume,
(nominal volume, volume, volume, volume, volume) actual, expected, actual, expected,
volume) actual, expected, actual, expected, VT (l) VT (l) VL (l) VL (l)
VT (l) VT (l) VL (l) VL (l) 30 l 35 69 20 42
30 l 35 51 20 31 100 l 100 455 75 274
100 l 100 117 75 71 280 l 299 Basis 180 Basis
280 l 299 Basis 180 Basis 800 l 852 754 600 454
800 l 852 905 600 545 1000 l 1000 1078 750 649
1000 l 1000 1100 750 661 1200 l 1271 1298 900 781
1200 l 1271 1304 900 785 1900 l 2044 2392 1500 1440
1900 l 2044 2086 1500 1256 19000 l 18887 7815 15000 4705
19000 l 18887 13216 15000 7956
b. Base case 30 l (laboratory scale)
b. Base case 30 l (laboratory scale) Scale Total Total Working Working
Scale Total Total Working Working (nominal volume, volume, volume, volume,
(nominal volume, volume, volume, volume, volume) actual, expected, actual, expected,
volume) actual, expected, actual, expected, VT (l) VT (l) VL (l) VL (l)
VT (l) VT (l) VL (l) VL (l) 30 l 35 Basis 20 Basis
30 l 35 Basis 20 Basis 100 l 100 231 75 132
100 l 100 81 75 46 280 l 299 152 180 87
280 l 299 206 180 118 800 l 852 382 600 218
800 l 852 624 600 357 1000 l 1000 547 750 312
1000 l 1000 758 750 433 1200 l 1271 658 900 376
1200 l 1271 900 900 514 1900 l 2044 1214 1500 693
1900 l 2044 1439 1500 822 19000 l 18887 3965 15000 2266
19000 l 18887 9120 15000 5211 Relationship: N2/N1 = DT1/DT2 = (VT1/VT2)1/3 = (VL2/VL1)1/3 (assumes geo-
Relationship: DT2/DT1 = (VT2/VT1)1/3 = (VL2/VL1)1/3. metric similarity).
peller tip speed increase (30), but the size of eddies does not TABLE 8. Scale-up based on constant power per unit volume
change (29). The Po/VL required to provide a certain OTR for Rushton radial flow impellers
generally decreases with scale (2). Scale-up on the basis of a. Base case 280 l (pilot scale)
constant Po/VL can result in a larger than necessary motor Scale Po/VL Po/VL Pg/VL Pg/VL
size. In addition, it is difficult to have high power per unit (nominal measured expected measured at expected at
volume inputs at the large scale (27) due to practical limita- volume) at Nmax at Nmax Nmax and Qmax Nmax and Qmax
(hp/1000 l) (hp/1000 l) (hp/1000 l) (hp/1000 l)
tions in motor size.
30 l NI 53.9 NI 42.4
Assuming geometrically similar vessels in which DT1/DT2
100 l NI 33.0 NI 26
= (VT1/VT2)1/3 (5), then scale-up based on constant ungassed 280 l 23.9 Basis 18.8 Basis
or gassed power per unit volume (Po/VL or Pg/VL, respec- 800 l 15.0 15.3 10.0 12.0
tively) simplifies to 1000 l 7.7 14.1 4.3 11.1
1200 l NA 13.2 NA 10.4
N2/N1 = (VT1/VT2)2/9 (5) 1900 l 13.9 10.9 6.8 8.6
This expression is very similar to N2/N1 = (VT1/VT2)1/3 used in 19000 l 4.4 4.65 2.0 3.7
Table 7 which was derived for scale-up on the basis of con- b. Base case 30 l installed hp (laboratory scale)
stant tip speed and geometric similarity (5). Although the Scale Po/VL Po/VL
gassing rate influence is incorporated into the value of Pg (nominal measured expected
based on measurements or expected decreases in power loss volume) at Nmax at Nmax
upon gassing, it can be challenging to accurately account for (hp/1000 l) (hp/1000 l)
the gassing (aeration) efficiency. In addition, this relation- 30 l NI Basis
ship is most effective for turbulent flows observed during 100 l NI 30.7
280 l 23.9 22.2
single cell E. coli and yeast cultures and less effective for
800 l 15.0 14.2
high viscosity mycelial cultures (5). 1000 l 7.7 13.1
As seen in Table 4, measured values of Pg/VL at maxi- 1200 l NA 12.2
mum aeration (Qmax) and agitation (Nmax) rates for stated 1900 l 13.9 10.1
working volumes ranged from nearly 19 hp/1000 l down to 19000 l 4.4 4.3
2 hp/1000 l as the scale increased from 280 l to 19,000 l. Relationship: (VL1/VL2)0.37 =(Po/VL)2/(Po/VL)1 or (Pg/VL)2/(Pg/VL)1. Mea-
Measured values of Po/VL were higher than those for Pg/VL sured Po and Pg values used in calculations except for 30 l base case
due to power decrease upon gassing, and the ratio of Pg/Po where installed value for Po of 1 hp used. NI, Power measuring device
not installed. NA, Calculation not applicable.
varied according to impeller type, fermentor scale and
sparger/impeller geometry (Table 5; 24). Tables 8a (for
Rushton radial flow impellers) and 9 (for Maxflo T and TABLE 9. Scale-up based on constant power per unit volume
A315 hydrofoil axial flow impellers) show that scale-up for hydrofoil axial flow impellers
based on measured Po/VL and measured Pg/VL values agreed
Base case 280 l (pilot scale)
reasonably well (within 26%) with expected values for the
800 l, 1900 l and 19,000 l scales. The notable exception was Scale Po/VL Po/VL Pg/VL Pg/VL
(nominal measured expected measured at expected at
the 19,000 l scale with Rushton impellers for which the ex- volume) at Nmax at Nmax Nmax and Qmax Nmax and Qmax
pected value was higher than the measured value by 85%. (hp/1000 l) (hp/1000 l) (hp/1000 l) (hp/1000 l)
Expected values for the 1000 l and 1200 l scale fermentors 30 l NI 42.6 NI 37.7
were notably higher by about 83180% due to the lower 100 l NI 26.1 NI 23.1
than typical measured Pg /VL for this scale vessel (versus 280 l 18.9 (M) Basis 16.7 (M) Basis
installed motor power). Measured values for the 30 l and 800 l 16.3 (M) 12.1 8.8 (M) 10.7
100 l scales were not able to be compared since no power 11.2 (A) 7.8 (A)
measurement device was installed. 1000 l 5.1 (A) 11.2 3.5 (A) 9.8
1200 l 10.1 (A) 10.4 6.8 (A) 9.2
Table 8b shows the use of installed values for Po/VL for 1900 l 10.0 (M) 8.6 8.0 (M) 7.6
the 30 l fermentor as a basis for scale-up. Agreement of the 19000 l 4.4 (M) 3.7 4.1 (M) 3.3
expected and actual values to within about 30% was evident 4.4 (A) 3.2 (A)
for all scales except the 1000 l scale which was higher by Relationship: (VL1/VL2)0.37 =(Po/VL)2/(Po/VL)1 or (Pg/VL)2/(Pg/VL)1. Mea-
70%. Using the 1000 l scale as a basis (data not shown), the sured Po and Pg values used in calculations. M, Maxflo T; A, A315.
expected values were lower for all scales by at least 40%, a
trend which is also due to the lower than typical measured For the maximum operating conditions of agitation (Table
Pg/VL. 1), impeller Reynolds numbers ranged from 0.488.8 106
Similar impeller Reynolds number (NRe) Scale-up for water (or for single cell E. coli and yeast broths with
can be accomplished based on a constant impeller Reynolds viscosities similar to water), suggesting that for filamentous
number, NRe: broths with higher viscosities flow may switch from turbu-
NRe = rNDI2/h (6) lent to laminar. The use of constant Reynolds number gen-
erally has not worked well for fermentation scale-up since
where h is the broth viscosity (8, 31). For the same broth, the effect of aeration on the process was not incorporated
this expression simplifies to (2), and the impeller Reynolds number generally increases
N2/N1 = (DI1/DI2)2 (7) for successful scale-up designs (26). Other dimensionless
TABLE 10. Comparison of typical heat up, hold time and cool down times as well as Fo and Ro values
for medium sterilizations as a function of scale
Heat up Hold Hold Cool down Fo Ro
Heat up Cool down
Scale (nominal volume/jacket type) time time time time total total
(area%) (area%)
(min) (min) (area%) (min) (min) (min)
100 l (dimple, jacket loop) 29 24.3 40 65.5 18.6 10.2 75.0 61.6
280 l (straight) 15.516.2 1516 40 74.9 2629.4 9.6 74.9 57.0
800 l (dimple) 2021 1315.6 45 74.378.6 17.718.6 8.210.0 73.7 63.6
1000 l (dimple, jacket loop) 3438 1920 45 7071 2727.5 910 108.8 74.1
1200 l (half pipe coil) 2430 1922 45 6566 3335 1214.5 85.4 66.2
1900 l (half pipe coil) 3542 2427 45 61.863.3 3032 1113 86.7 72.8
19000 l (half pipe coil) 8388 37 45 46.4 95110 16.4 91.2 86.6
Medium hold temperature of 123.5C for batch sterilization. Hold temperatures of 124C for 1000 l and 123C for 100 l scale. Fo and Ro values
calculated according to Junker et al. (38). Only temperatures above 60C were included in summation. Heat up and cool down times calculated
from 40C. A 19,000 l scale vessel used cooling tower water for cool down and not chilled water. Area% is the area under the temperature versus
time curve for the stage divided by the total area. Heat up and cool down area percentages calculated for temperatures above 60C.
groups also have been examined for scale-up with limited scale-up, but mainly between the pilot scale and production
success, often resulting in technically unrealistic equipment stages. Most commonly when the power is changed only by
and operating parameters. As it is difficult to maintain all increasing agitation speed, then Eq. 9c simplifies to
dimensionless parameters constant upon scale-up, those most
KLa = f2(Pg/VL)0.50 for production vessels (33) (9d)
important to the process must be identified accurately.
Constant oxygen uptake rate (OUR), mass transfer In laboratory scale fermentors where measurements of Pg/VL
coefficient (KLa) or dissolved oxygen (DO) Scale-up are difficult to accurately obtain, then the key components
based on constant OUR assumes that the OUR is equal to of the power number (N, DI) may be used:
the OTR:
KLa = f2(N 3DI2)0.42 for laboratory vessels (34) (9e)
OTR = KLa(Csat - CL) = OUR = mX/YX/O2 (8)
where, although the exponent of 0.42 was established for
where Csat is the broth DO concentration at saturation, CL is a 0.6 l working volume, the literature range is 0.160.68.
the measured broth DO concentration, m is the specific Since they are generally most applicable at or near the con-
growth rate, X is the measured cell density and YX/O2 is the ditions used to determine the exponents, these correlations
calculated cell yield per amount of oxygen consumed (32). might best be used for only qualitative guidance in scale-up
Changes in back-pressure and hydrostatic pressure with calculations (28).
scale-up influence the values of Csat (and subsequently CL). As shown in Table 5, calculated values of (Pg/VL)aVsb
It is also possible to use the log mean of the DO concentra- using measured values of Pg/VL and Eq. 9a and 9b are
tion difference. Since for most aerobic fermentations the reasonably similar (average [ave]: 7.8 1.9; relative stan-
critical DO concentration which adversely affects growth dard deviation [rsd]: 24%) from the 280 l to 19,000 l (180 l
rate is very low, CL is assumed to be zero. 15,000 l working volume) scales. When design values of
Several correlations of the general form Po/VL are used, much higher values of (Pg/VL)aVsb are ob-
tained as expected, with the values being reasonably similar
KLa = f2(Pg/VL)aVsb (9)
(ave: 11.0 2.2; rsd: 20%) from the 800 l to 19,000 l scales
exist to estimate KLa using gassed power per liquid volume, and much higher below the 800 l scale (600 l working vol-
Pg/VL , and gas superficial velocity, Vs, for fermentations ume). Only a fraction of these design values actually can be
(similar to the Van Riet correlation for mass transfer): delivered to the fermentation broth with the amount depen-
dent on vessel/agitator geometry, rheology, agitator speed,
KLa = f2(Pg/VL)0.95Vs0.67 and superficial velocity (28).
for laboratory scale (8 l) vessels (5) (9a) From a survey of industrial fermentors up to 100,000 l
in volume, KLa values ranged from 400800 h1 (Einsele,
KLa = f2(Pg/VL)0.67Vs0.67 Abstr. 5th Intern. Ferment. Symp., 1976). The KLa values
for pilot scale (400 l) vessels (5) (9b) obtained in Tables 11 and 12 are generally within this range
assuming a Henrys law constant of 1 mmol/l-atm. The KLa
KLa = f2(Pg/VL)0.50Vs0.50 varies roughly with the inverse of the apparent broth viscos-
for production (23,000 l46,000 l) vessels (5) (9c) ity (15). Surface aeration can be a substantial contributor for
smaller-scale fermentors, specifically about 33% for 5 l ves-
where f2 is a proportionality constant in all equations whose sels and about 10% for 50 l vessels (15). Pilot scale fermen-
value varies depending upon the specific process and the tors below 250 l in volume usually have significant surface
units of KLa, Pg/VL and Vs used in the calculations. All vol- aeration compared to larger scale vessels, so it is generally
umes cited in Eq. 9ac are operating volumes. For these best to scale-up from larger vessels of about 500 l1000 l
correlations, the dependence of KLa on Pg/VL is lower as the (8). Surface aeration decreases markedly with scale (27);
vessel scale increases (i.e., the exponent decreases). Simi- thus for larger vessels, KLa values can be more easily inter-
larly, the dependence of KLa on Vs also decreases upon preted. Scale-up based on KLa is complicated by the fact
TABLE 11a. Representative historical (1992 through mid-2001) comparison of achievable processing conditions
as a function of scale for E. coli cultivations
Peak oxygen Air flow Impeller Gassed Calculated Value of f2
Fermentation
Cultivation/Scale uptake rate, Pressure speed, power, Pg/VL KLa at using Eq. 9b
volume (l)
(nominal volume) rate Q (kg/cm2) N Pg (hp/1000 l) peak OUR KLa/[(Pg/VL)0.67
(impeller type)
(mmol/l-h) (l/min) (rpm) (hp) (mmol/l-h-atm) (Vs)0.67]
E. coli DH5/280 l 180 (R) 260 300 1.8 400 NI NI 685 NA
E. coli DH5/280 l 150 (M) 172 190 1.25 400 NI NI 624 NA
E. coli PF436/280 l 175 (M) 65 80 0.6 383 NI NI 346 NA
E. coli RR1/280 l 160 (M) 77 80 0.3 409 NI NI 472 NA
E. coli OP50/280 l 175 (R) 39 100 0.5 213 NI NI 186 NA
E coli K12/800 l 605 (M) 94 400 0.7 287 6.3 10.4 434 76
E. coli DH5/1000 l 600 (M) 141 600 1.0 300 4.1 6.8 738 143
E. coli PF436/1900 l 800 (M) 38 400 0.7 178 5.6 7.0 167 55
E. coli RR1/1900 l 760 (M) 95 450 0.3 229 11.2 14.7 596 111
E. coli OP50/1900 l 810 (R) 49 500 0.7 125 2.7 3.3 303 143
E. coli Polym./1900 l 1080 (M) 101 600 1.2 225 9.0 8.3 486 110
P. aeruginosa/1900 l 1200 (M) 47 510 0.3 132 7.4 6.2 186 57
Values bolded are at/near (within 20%) of maximum conditions for that particular scale. R, Rushton; M, Maxflo T; A, A315. NI, Power measure-
ment device was not installed. NA, Calculation not applicable.
TABLE 11b. Representative historical (1992 through mid-2001) comparison of achievable processing conditions
as a function of scale for yeast cultivations
Fermentation
Cultivation/Scale uptake rate, Pressure speed, power, Pg/VL KLa at using Eq. 9b
volume (l)
(nominal volume) rate Q 2
(kg/cm ) N Pg (hp/1000 l) peak OUR KLa/[(Pg/VL)0.67
(impeller type)
C. sorbophila/280 l 150 (R) 54 100 0.7 223 NI NI 226 NA
C. chilensis/280 l 180 (R) 141 180 1.5 400 NI NI 297 NA
S. cerevisiae QC2B/280 l 180 (R) 74 80 0.7 354 NI NI 350 NA
S. cerevisiae 1375/280 l 180 (R) 64 90 0.5 315 NI NI 324 NA
C. sorbophila/800 l 475 (R) 105 505 0.7 320 >7.5* >15.8 465 NA
475 (M) 90 475 0.7 286 >7.5* >15.8 386 NA
C. chilensis/800 l 600 (R) 106 335 1.2 245 4.2 7.7 325 77
500 (M) 117 490 1.7 220 3.2 7.0 318 62
S. cerevisiae QC2B/800 l 570 (M) 93 220 0.7 265 2.4 4.2 463 218
S. cerevisiae 1375/800 l 530 (R) 63 250 0.5 266 5.2 9.8 344 84
S. cerevisiae 1375/1000 l 600 (M) 60 400 0.34 308 4.2 7.0 844 211
C. chilensis/1900 l 1500 (M) 49 530 0.83 175 3.1 2.1 252 155
S. cerevisiae 1375/1900 l 1400 (M) 53 700 0.5 173 5.5 3.9 264 89
Values bolded are at/near (within 20%) of maximum conditions. Values marked with an asterisk denote saturated power measurement readings.
R, Rushton; M, Maxflo T; A, A315. NI, Power measurement device was not installed. NA, Calculation not applicable.
that it is process-specific and that it changes over the course Constant gas flow number (NA), volumetric gas flow
of the fermentation (35), making it difficult to reliably quan- rate per unit volume of liquid (vvm or Q/VL), or superfi-
tify. cial velocity (Vs) Scale-up also can be performed based
Alternatively, an optimal value for CL may be determined on the flow (aeration) number, NA = Q/NDI3, where Q is the
from laboratory studies and used for scale-up (2). Equation volumetric flow rate. A typical range for the flow number
8 then can be rearranged to calculate KLa values during the for production fermentors is 0.10.15 (29) which compares
fermentation at various ages. Scale-up based on constant favorably with the values of 0.120.13 for the 19,000 l fer-
DO can be an attractive method. Although KLa and OUR mentors with hydrofoil impellers and is much lower than
can change dramatically over the course of the fermenta- the value of 0.3 obtained for the 19,000 l fermentor with a
tion, the minimum acceptable value of CL is usually known Rushton impeller (Table 4). Aeration numbers for other
from laboratory studies. A CL above 3070% saturation pilot scale vessels (100 l1900 l) ranged from 0.0270.14
usually assures adequate DO in less mixed regions of a vis- with an aeration number of 0.032 obtained for the 30 l labo-
cous mycelial fermentation; for a less viscous E. coli or ratory vessel (Table 4).
yeast fermentation, a CL above a lower limit of 1030% sat- Scale-up based on the volumetric gas flow rate per unit
uration can be adequate. Scale-up based on constant DO volume of liquid (Q/VL or vvm) also should be examined to
must consider the scale-up of methods to control DO such ensure that resulting values of superficial velocity are rea-
as agitation, pressure and air flow rate (19). Cascade control sonable. For a specific process, a balance must be achieved.
of DO by agitation, pressure and air flow rate can be effec- If the volumetric gas flow rate per unit volume of liquid,
tive in maintaining DO above critical values (35). Q/VL, remains constant upon scale-up, then Vs may increase
to the point of flooding in production-scale tanks (2). Simi-
TABLE 12a. Comparison of recent (mid-2001 to 2002) typical achievable processing conditions as a function of scale for E. coli cultivations
Air flow Impeller Gassed Calculated Value of f2
Scale Fermentation Peak
rate, Pressure speed, power Pg/VL KLa at using Eq. 9b
(nominal volume (l) OUR
Q (kg/cm2) N Pg (hp/1000 l) peak OUR KLa/[(Pg/VL)0.67
volume) (impeller type) (mmol/l-h)
(l/min) (rpm) (hp) (mmol/l-h-atm) (Vs)0.67]
280 l 180 (R) 155 300 1.2 460 3.25 18.1 572 51
180 (M) 158 300 1.2 460 3.4 18.9 475 41
800 l 600 (R) 142 500 1.4 330 9.2 15.3 391 46
600 (M) 115 500 1.5 330 9.2 15.3 354 42
600 (A) 126 470 1.5 330 6.2 10.3 330 40
600 (HE) 127 500 1.2 338 8.6 14.3 393 48
600 (MC) 124 500 1.2 338 9.0 15.0 364 40
600 (CC) 136 500 1.25 330 7.2 12.0 527 70
1200 l 900 (A) 116 1200 1.3 280 5.5 6.1 296 42
1900 l 1500 (R) 96 1500 1.0 230 11.4 7.6 354 46
1500 (A) 116 1500 0.9 230 13.2 8.8 465 55
Values bolded are at/near (within 20%) of maximum conditions for that scale. R, Rushton; M, Maxflo T; A, A315; HE, HE-3/Maxflo T; MC,
Maxflo T/CD-6; CC, CD-6/CD-6.
TABLE 12b. Comparison of recent (mid-2001 to 2002) typical achievable processing conditions as a function of scale for yeast cultivations
Scale Fermentation
uptake rate, Pressure speed, power, Pg/VL KLa at using Eq. 9b
(nominal volume (l)
rate Q (kg/cm2) N Pg (hp/1000 l) peak OUR KLa/[(Pg/VL)0.67
volume) (Impeller type)
280 l 180 (M) 98 235 1.0 338 1.7 9.6 430 69
800 l 600 (R) 93 500 0.7 325 7.7 12.8 453 60
500 (M) 97 268 1.1 276 5.0 9.9 490 114
600 (A) 82 500 0.7 327 5.0 8.3 577 101
600 (MC) 92 500 0.7 271 4.6 7.7 461 85
1200 l 900 (A) 94 1000 1.1 226 2.8 3.1 390 99
1900 l 1500 (R) 79 925 0.97 172 5.0 3.3 385 120
1500 (M) 88 980 0.97 170 6.0 4.0 450 119
19000 l 14600 (M) 78 7800 0.89 96 16.2 1.1 380 136
14600 (A) 82 9300 0.95 106 16.2 1.1 343 109
14600 (R) 74 8400 0.90 115 29.5 2.0 343 78
Values bolded are at/near (within 20%) of maximum conditions for that scale. R, Rushton; M, Maxflo T; A, A315; HE, HE-3/Maxflo T; MC,
Maxflo T/CD-6; CC, CD-6/CD-6.
larly, if it is desired to maintain Vs constant upon scale-up, accomplished by maintaining estimated mixing times con-
then larger values of Q/VL must be implemented at the stant. Several relationships have been derived or empirically
smaller scale (36). Typical values of Q/VL range from 1.67 developed
down to 1.0, with the values generally decreasing at the
Tmix = f3VL0.3 (10a)
larger scale (Table 4). Although the volumetric air flow rate
has relatively little effect on the KLa value, higher air flow from a survey of industrial fermentors from 50 l to 100,000 l
rates can cause dramatic foaming (27) and higher gas holdup in volume (26; Einsele, Abstr. 5th Intern. Ferment. Symp.,
in the fermentor. If the superficial velocity, Vs, and Pg/VL are 1976) and
constant, the gas holdup does not change with scale-up (29).
Tmix = f3(Pg/VL)0.37 (10b)
Flooding happens when the superficial air velocity, Vs,
approaches 2550% of the bubble rise velocity since the for a tetracycline process up to 52,000 l in volume (Einsele,
fermentor gas holdup volume only can be about 20% or less Abstr. 5th Intern. Ferment. Symp., 1976), where k is a pro-
(15). In the case of water with an average bubble rise ve- portionality constant in both equations. For geometrically
locity of 22 cm/s, flooding occurs at 510 cm/s (15). When similar vessels in the region of turbulent flow:
flooding occurs, the impeller cannot disperse all the sup-
Tmix N 2/3DI1/6 = constant (5) (10c)
plied gas, the gas rises as big bubbles to the liquid surface
and the impeller pumping action diminishes (2). As shown Thus, solving Eq. 10c assuming equal mixing times gives
in Table 5, Vs ranges from 0.663.4 cm/s for vessels be- Eq. 10d (5):
tween 30 l and 1900 l in total volume, jumping to 8.1 cm/s
N2/N1 = (DI2/DI1)1/4 (10d)
for the 19,000 l scale. Based on these guidelines, possibly
the 19,000 l scale Qmax conditions may be prone to flooding. and the corresponding power inputs are given by Eq. 10e
Note that flooding also may occur at low agitation speeds (5):
with too high of an air flow rate for all scales.
(Po/VL)2/(Po/VL) 1 = (N23DI22)/(N13DI12) (10e)
Constant mixing time Alternatively, scale-up can be
For geometrically similar vessels in the region of turbulent

flow where both Po/VL and mixing time are constant, Eq.
10e becomes (12)
N1/N2 = (DI2/DI1)2/3 (10f)
The volumetric power input required to maintain equal mix-
ing time increases as VL2/3. Thus, using the relationship of
Eq. 10f, Pg/VL can become prohibitively high upon scale-up
and is usually overestimated. This technique generally has
not worked well for fermentations (2).
A mixedness index, Im, also has been proposed (7) which
does not assume geometric similarity:
Im = f3(ITS)(DT/HT)(DT)2/3 (10g)
This expression may be particularly useful for scale-up for
vessels already constructed in which geometric similarity FIG. 3. Linear regression of literature mixing times (Eq. 10h) re-
ported for laboratory, pilot scale and production processes (4, 14, 20).
may not have been maintained. Mixing times need to be
evaluated relative to nutrient mass transfer rates for fed-
batch cultures in the presence of cellular nutrient uptake. ported (14). Finally, mixing times of 15 s for 120 l, 40 s for
For a culture (not specified but likely to be a yeast) with a 1200 l and 60 s for 12,000 l vessels have been reported (20).
cell density of 20 g/l growing at a rate of 0.2 h1 (doubling These mixing times were reported for both Newtonian and
time of 3.5 h), if the DO (CL) is at 20% saturation, oxygen in non-Newtonian fluids/broths.
the broth would be depleted in 2.5 s (32). In the case where These mixing time estimates may be graphed (Fig. 3).
glucose was the limiting nutrient, glucose could be depleted Linear regression of these available data points from the lit-
as fast as 4.5 s (32). Longer mixing times can cause locally erature yields the equation
high glucose rates which in turn can cause locally low DO
Tmix = 17.5 log10 (VL) - 19.4
levels owing to higher cell metabolism. As a consequence,
local areas of mixed acid E. coli fermentations can result, (10 l to 60,000 l, r 2 = 0.876) (10h)
producing overall lower biomass yields upon scale-up (9). Tmix = 223.5 log10 (VL) - 1004.6
Thus, scale-up based on mixing time can be relevant for
(60,000 l to 120,000 l, r 2 = 0.902) (10i)
fed-batch E. coli and yeast cultures, especially at high cell
densities. where Tmix is the mixing time in seconds and VL is the liquid
The characteristic time analysis above can be extended working volume in liters. Clearly the mixing time increase
further and divided into characteristic times for transport with volume is steeper once the working volume is above
phenomena (transfer or supply) and characteristic times for 60,000 l. Equation 10 h was used to estimate mixing times
conversion (consumption or reaction) rates (11). Transport for each existing fermentor scale (Table 4). The relative
phenomena include oxygen transfer (including oxygen trans- magnitudes of these times can be compared with those ob-
fer from the gas bubble to the liquid), liquid circulation, gas tained from the times estimated using Eq. 10a and 10b as-
residence, and heat transfer. Conversion rates include the suming the proportionality constant, f3, remains constant
zero and first order rates for oxygen and substrate consump- with scale.
tion, cell growth and heat production. Other influences After the initial strategies outlined
It can be important to compare nutrient consumption and above are implemented, the resulting vessel design needs to
transfer rates with each other as well as with circulation consider other influences to assure optimal performance.
times to establish whether gradients are likely to exist (11). Heat transfer rates Heat evolution is the combination
Specifically, for gluconic acid fermentation in a stirred tank of mechanical heat from the agitator and metabolic heat
by a fungal culture, oxygen limitation can occur if con- from the culture. The ratio of metabolic heat evolution to
sumption and transfer rates are similar in magnitude. If liq- oxygen consumption is approximately 115 kcal heat evolved
uid circulation times also are this same order of magnitude, per mole of oxygen consumed for selected E. coli, yeast and
then oxygen gradients are favored. In contrast, temperature fungal cultures (32, 37). The total amount of oxygen con-
gradients are less likely to occur since, although heat pro- sumed by the culture can be estimated by integration of the
duction and transfer rates are similar, they often are substan- OUR value versus time curve then multiplication by the
tially greater than liquid circulation times. This analysis is tank working volume. The desired heat transfer coefficient
applicable to high cell density fed-batch E. coli and yeast and jacket area then can be evaluated using expected cool-
cultures. ing fluid flow rates and inlet/outlet temperatures. Require-
Observed mixing times of several seconds exist for labo- ments for the jacket type (e.g., dimple, half-coil) and jacket
ratory fermentors, 2030 s for 10002000 l pilot scale fer- area then are established. For large fermentors over 5000 l,
mentors and 70140 s for 60,000 l120,000 l production fer- it can be difficult to sustain OURs above 300 mmol/l-h since
mentors (4). Specific mixing times for these scales of 5 s for heat transfer problems arise.
10 l, 20 s for 1000 l, 29 s for 1800 l, 67 s for 60,000 l, 100 s Medium sterilization effects As the fermentor scale in-
for 100,000 l and 140 s for 120,000 l vessels have been re- creases, the heat up and cool down times become a larger
proportion of the overall sterilization time cycle as shown in from Pg/VL and KLa correlations.
Table 10. The heat up time portion increases from about An application of this method is the use of KLa for scal-
15% to about 37%, and the cool down portion increases ing-up a Bacillus thuringiensis fermentation. This scale-up
from 10% to 16% as the scale rises from 280 l to 19,000 l. was accomplished using the equation, KLa = constant N aVsb
The 100 l and 1000 l scales are exceptions to this trend as (obtained by combining Eq. 9, the expected ratio of Pg/VL,
they required slightly longer than the expected ranges be- and Eq. 3) with scale-up on the basis of KLaPT where PT is
cause they are equipped with a recirculating jacket loop the total pressure in the vessel including head pressure (40).
with indirect heating and cooling via heat exchangers. The Another application is to use an iterative strategy based on
values of Fo increased from about 75 to about 91 min and incremental air flow rates to calculate resulting scale-up pa-
the values of Ro increased from about 57 to about 87 min rameters and then to examine each set of parameters for a
over this same range of scales (Table 10; 38). These in- particular flow rate to further optimize compressor and agi-
creases in Fo and Ro directly translate to a rise in the level of tator power requirements (36).
sterilization overkill and medium heat stress respectively as Method of Ju and Chase/Diaz and Acedevo This
scale increases. The adverse impact of medium heat stress is method (2, 41) focuses on scaling-up based on equivalent
process dependent and can be minimized with the use of OTR not KLa. First, the scale-up volume is selected, then
continuous (high temperature, short time) media steriliza- geometric similarity is used to obtain DT. Constant impeller
tion. tip speed is assumed to obtain N. Using the relationship,
Biological factors Biological factors, such as the num- Pg/VL = f1VLc (Eq. 4), Pg/VL then is estimated and, using em-
ber of generations through which the organism will progress pirical relationships between Pg/VL and KLa (Eq. 9ac), the
over the course of the seed and production fermentations, KLa values for the scale-up fermentor are determined. Final-
need to be considered in the selection of the final production ly, the OTR rate for the large fermentor is matched with that
scale. Assuming exponential growth, the number of genera- of the small scale fermentor and the back-pressure for the
tions, Ng, can be expressed as (12) large fermentor is calculated assuming CL is 0 mmol/l.
The key element of this method is that there are three de-
Ng = 1.44 (lnVL + ln XN - ln XNo) (11)
grees of freedom for scale-up. These are commonly N, Q
where XN is the final cell number (or mass) and XNo is the and DI/DT (i.e., reactor geometry). Thus, only three items
initial inoculum cell number (or mass). The stability of the may be specified to be constant for scale-up. If another de-
recombinant DNA insert and the requirement for an agent to gree of freedom is added such as the gas phase partial pres-
exert selective pressure need to be evaluated for the number sure, then this value also can be specified to maintain the
of expected generations in the process plus a comfortable maximum OTR constant. To determine the effect on the cul-
safety margin. tivation, it is generally useful to run small scale fermenta-
Generalized approaches to scale-up Several authors tions using gas blending to vary this inlet oxygen partial
have recommended approaches or combinations of ap- pressure.
proaches to scale-up based on the equations and principals Method of Wang et al. In this method (42), two key
described above. No single method appears to be suitable values are maintained constant on scale-up: KLa (calculated
for all fermentations with a high probability of success (5), by Eq. 9ac) and ITS. The ratio of DI/DT then is adjusted to
and the applicability of one method over another is process- within reasonable limits to complete the design. Although
specific. Success often depends on the reliability of empiri- geometric similarity is not maintained, the resulting varia-
cal scale-up correlations and the integrity of small-scale tion of the DI/DT ratio with scale often can still provide ade-
data. A few examples are highlighted below. quate gas dispersion. This technique adds flexibility for in-
Method of Hubbard This method (39) was developed stallations of existing fermentors.
as a combination of approaches from other authors. During Proposals for improved scale-up calculations This
the laboratory scale fermentation, air flow rate, impeller simplified method (27) evaluates key quantities of scale-up
speed, yield, and fermentor geometric dimensions are mea- interest based on two variables: N and DI. The impeller
sured. Basic broth properties such as density, viscosity, sur- Reynolds number is represented by NDI2, the Froude num-
face tension, and oxygen diffusion coefficient are deter- ber by N 2DI, the Weber number by N 2DI3, the gassed power
mined. (Of these broth properties, it is probably most im- per unit liquid volume by N 3DI2, the impeller tip speed by
portant to understand the broth rheological behavior for NDI, and Q/HT by DI/N (where HT is specifically the height
mycelial cultures.) Several quantities, such as Q/VL, NRe, of the fermentor and not the height of the liquid volume). It
ITS, and NA, are calculated from the laboratory scale fer- combines relevant dimensionless group analysis with other
mentor conditions based on measured quantities. empirically applicable parameters.
For the plant scale fermentor, a volume is selected based Scale-up analysis using one or more of these above meth-
on product yield and plant capacity. Geometric similarity ods has suggested methods for operating laboratory fermen-
then is used to calculate vessel dimensions. Scale-up is tors for the best scale-down performance. For example,
based on matching KLa values and then proceeding in either nitrogen-diluted air is recommended to be used at the 10 l
one of two ways. The first way is to calculate the flow rate, scale to appropriately mimic scale-up to the 10,000 l scale
Q, by either holding Q/VL or superficial velocity, Vs, con- (2). Scale-down studies designed to simulate large-scale
stant, then to calculate the impeller speed, N, based on Pg/VL operating conditions have been highly successful in some
versus KLa correlations (Eq. 9ac). The second way is to set cases in predicting behavior and identifying causes for sub-
N using constant impeller tip speed, then to calculate Q optimal large-scale performance (4346).
Current scale-up practices for E. coli and yeast cultures III. SCALE-UP RESULTS FOR
are largely based on maintaining equivalent CL, KLa or OTR PRIOR FERMENTATIONS
performance as a first pass. In these fermentations, oxygen
(1992 THROUGH MID-2001)
supply is limiting upon scale-up due to high cellular oxygen
demand and not due to high broth viscosity as in the case of A survey of processing was conducted in this fermenta-
fungal cultures. Subsequently an evaluation of the impact of tion pilot plant from 1992 through mid-2001 to obtain in-
mixing time as it affects DO and nutrient distribution can be formation about achievable process conditions for E. coli
conducted, which is especially recommended for high cell (Table 11a) and yeast (Table 11b) fermentations. Bolded
density fed-batch cultures. values represent operation within 20% of maximum condi-
tions for agitation and aeration for the pilot plant fermentors
shown in Table 1. In the case of fermentor back-pressure,
II. FERMENTATION PROCESS CONDITIONS
the desired maximum value was fixed at 1.5 kg/cm2, although
To evaluate the operating performance of existing pilot during this period of operation (early 1990s) some fermen-
scale vessels, fermentor conditions (working volume, air tations were conducted at pressures as high as 1.8 kg/cm2,
flow rate, pressure, impeller speed, gassed power draw, a back-pressure subsequently found to adversely affect the
mass transfer coefficient, OUR) were compiled based on agitator double mechanical seal longevity. Also during this
historical records for several E. coli (Table 11a) and yeast period, power draw readings were not available at 280 l
cultures (Table 11b). OUR was calculated based on mea- scale and the watt transducers installed at 800 l scale, which
surements of off-gas composition by a mass spectrometer were not corrected for gearbox losses (24), became satu-
(47). Data was taken at the time of peak OUR which did not rated at higher power draws.
necessarily correspond to the time of peak mass transfer co- Table 11a illustrates that historical E. coli cultivations
efficient. Cultivations were conducted at the 280 l to 1900 l predominantly challenged the maximum impeller speed pri-
scales over the past decade. In addition, specific recent stud- marily at the 280 l and 1000 l scales. Only a few 280 l cul-
ies were performed at the various scales (280 l19,000 l) for tivations simultaneously approached peak conditions of air
one example E. coli (E. coli DH5, Table 12a) and one ex- flow rate, agitation and pressure. Peak OURs ranged from
ample yeast process (Candida chilensis, Table 12b) using 38 to 260 mmol/l-h with OURs above 90 mmol/l-h reached
fermentation media designed to promote high-peak OTR. for each of the four scales tested. Pg/VL and KLa values cal-
Tabulated data are representative of typical fermentations of culated at peak OUR ranged from 3.314.7 hp/1000 l and
that specific process at that selected scale. 167738 mmol/l-h-atm, respectively. Although there was
Control parameters for each fermentation varied accord- extensive experience at the 280 l and 1000 l scales with high
ing to development objectives. After its initial decline from OUR fermentations, the degree of challenge to the operating
pre-inoculation levels, DO was generally controlled be- capacity of the vessels at the other scales was limited. KLa
tween 30% and 80% of saturation, calibrated to air at am- values achieved at the smaller 280 l scale were generally
bient pressure, using various strategies. In some cases, the achievable upon scale-up to the 1000 l or 1900 l scales for
fermentation was initiated with the agitation, back-pressure those processes for which this was a development goal (E.
and/or air flow rates in cascade control with DO. In other coli DH5, E. coli RR1). Values of the proportionality con-
cases, when the need to control DO at its set point resulted stant, f2, from Eq. 9b ranged from 55 to 143, indicating an
in the agitation and air flow rates reaching maximum set- expected variability in performance of any empirical scale-
tings, these two parameters were placed in automatic mode up correlation due to the specific process, scale-up and op-
at their maximum set points and then back-pressure was erating parameters.
placed in cascade control. Other strategies were utilized de- Table 11b summarizes comparable historical data for yeast
pending on the specific process requirements. For example, cultivations. As noted in the case of the E. coli processing,
if foaming occurred in the fermentation or a higher dCO2 few challenges to peak operating conditions were made ex-
concentration was desired, the back-pressure was typically cept at the 280 l and 1000 l scales. Peak OURs were notably
raised to 11.5 kg/cm2 earlier in the process. lower than in the case of the E. coli fermentations, ranging
Specific process descriptions have been published for from 49 to 141 mmol/l-h with OURs above 50 mmol/l-h
some of the processes described (E. coli RR1 [48, 49], E. reached for each of the four scales tested. Pg/VL and KLa
coli OP-50 [50], E. coli PF436 [51], Saccharomyces cere- values calculated at peak OUR ranged from 2.1 hp/1000 l
visiae QC2B [52], S. cerevisiae 1375 [53], Pseudomonas to over 15 hp/1000 l and 226844 mmol/l-h-atm, respective-
aeruginosa MB5001 [54], and Candida sorbophila [5557]). ly. These ranges were similar to those noted for E. coli proc-
Other process descriptions are not published (E. coli DNA esses. Again the extensive experience at the 280 l and 1000 l
polymerase, E. coli K12, E. coli DH5, C. chilensis), but are scales was not matched at the other scales. In the case of
consistent with current state-of-the-art procedures. Exact these yeast processes (C. sorbophila, C. chilensis, and S.
processes run were based on these descriptions, but they de- cerevisiae 1375), the KLa values achieved at the 280 l scale
viated significantly in many cases to achieve process devel- were generally able to be obtained at the larger 800 l, 1000 l
opment goals. and 1900 l scales. Values of the proportionality constant, f2,
from Eq. 9b generally ranged from 62 to 218, again indicat-
ing expected variability in performance due to the process,
scale-up and operating parameters. For a specific process at
a specific scale, the range was substantially smaller.
conditions from typical process development data sets. Often

IV. SCALE-UP RESULTS FOR CURRENT STUDIES
the range of process conditions that is needed conflicts with
Based on this historical analysis of process performance, how to optimally execute the processes, making data diffi-
recent studies (mid-2001 to present) were conducted to im- cult to obtain and back-calculate. It can be difficult to vary
prove the challenge to fermentor peak operating conditions conditions within a single cultivation as was done previous-
for E. coli and yeast fermentations. In the case of E. coli ly (58) without adversely affecting subsequent data. Conse-
fermentations, initial carbon and nitrogen concentrations quently, not all processes/scales were able to be analyzed if
were raised to increase the peak OUR beyond that which the operating conditions at peak OUR values for individual
might normally be observed with this process. It was de- cultivations did not vary sufficiently.
sired to conduct specific studies at the 800 l, 1200 l, 1900 l Table 13a summarizes the relationship between peak OUR
and 19,000 l scales to obtain more complete information and KLa:
about the capabilities of the installed pilot scale equipment.
OUR = A1KLa + B1 (12a)
Upgraded variable frequency drives (VFDs) were installed
on all, but the 19,000 l scale vessels (which retained their for selected historical and current processes at various scales
watt transducers) in which the power draw was monitored for which the broth DO levels were similar. The slope, A1,
directly from the VFD electrical current (Altivair 66; varies from 0.075 to 0.46, indicating a large dependence on
Schneider Electric, Palatine, IL, USA) This resulted in the process and operating conditions on mass transfer. For a
new capability to measure power draw at the 280 l scale and specific process, however, the values when attainable were
an expanded measurement range for the 800 l scale. reasonably constant upon scale-up.
Table 12a summarizes the achievable processing condi- Prior scale-up studies in pilot scale vessels have been
tions for the E. coli DH5 process for a process scaled-up based on secondary metabolite fermentations in which gen-
based on maintaining similar minimum DO levels. For these eral agreement was found with established KLa and Pg/VL
aerobic processes, DO was required to be above its critical trends (58). Since the more recent focus of pilot plant stud-
value to maximize growth and productivity. Peak OURs de- ies has been on scale-up of E. coli and yeast cultures, peak
creased slightly from about 155158 mmol/l-h to about 96 data from recent scale-up studies have been analyzed and
116 mmol/l-h upon scale-up from the 280 l to 1900 l scales. results presented in Table 13b. The exponent of Pg/VL in Eq.
Pg/VL decreased with scale as expected ranging from about 9b, A2, was calculated for selected historical and current
1819 hp/1000 l at the 280 l scale to 6.18.8 hp/1000 l at the processes at various scales according to
1200 l and 1900 l scales. Calculated KLa values declined
log KLa = A2 log(Pg/VL) + B2 (12b)
only slightly with scale, decreasing from 475572 mmol/l-
h-atm at the 280 l scale to 354465 mmol/l-h-atm at the The values obtained appear to be consistent for both E. coli
1900 l scale. Values of f2 in Eq. 9b were substantially more and yeast processes and are about 0.960.98, compared with
uniform than found with the historical data, ranging from 40 0.580.8 found previously for a filamentous bacterial and a
to 70, matching the lower range found with the historical fungal cultivation (23, 58). The higher values reflect the
E. coli process data. Values were relatively consistent with greater impact of a KLa change with OUR for these E. coli
scale and operating conditions, suggesting a reliable empiri- and yeast cultures, most likely due to their lower broth vis-
cal relationship may be obtainable. cosity and largely single cell morphology. Interestingly, the
Achievable processing conditions for the yeast C. chilen- higher value of the exponent appears to be more consistent
sis process are summarized in Table 12b, again based on with the laboratory scale correlation (Eq. 9a) than the pilot
scaling-up using similar minimum DO levels. Upon scale- scale correlation (Eq. 9b).
up from the 280 l to 19,000 l scale, peak OURs decreased For mycelial broths, rheological characteristics influence
slightly from about 98 mmol/l-h to about 7482 mmol/l-h. scale-up performance. Heat and oxygen transfer rates are
As expected, Pg/VL decreased with scale ranging from about 550% of bacterial fermentations and bulk mixing is poorer
9.6 hp/1000 l at the 280 l scale to 1.12.0 hp/1000 l at the leading to lower broth homogeneity (28). As a consequence,
19,000 l scales. Both peak OUR and Pg/VL values were no- ITS often has been a useful rule of thumb for scale-up (27).
tably lower for the yeast process than for the E. coli process. Rheology is less important for single cell bacterial and yeast
Calculated KLa values declined only slightly with scale, de- fermentations compared with the relative magnitudes of nu-
creasing from about 430 mmol/l-h-atm at the 280 l scale to trient uptake and supply rates. Thus, scale-up based on DO,
343380 mmol/l-h-atm at the 19,000 l scale. Values of f2 in OUR or KLa often has been more useful for these cultiva-
Eq. 9b ranged from 60 to 136 and were less uniform with tions. For facilities with existing installed equipment, relia-
scale and operating conditions than found with current E. ble scale-up is most readily achieved based on selecting op-
coli process data. This difference may have been due to the erating conditions such that the minimum DO remains simi-
tendency of this culture to clump and even branch during lar between the two scales. Implications for other key pa-
growth. The range of f2 values also was lower than that rameters such as OUR and KLa then can be easily evaluated.
found with the yeast historical data. Owing to the availability of recombinant E. coli and yeast
cultures with high specific productivities, typical production
volumes for recombinant proteins often do not range above
V. TRENDS AND IMPLICATIONS FOR SCALE-UP
5000 l and/or may not require high cell density processes.
Established relationships for scale-up can be difficult to As demand for capacity increases, additional efforts may be
use due to lack of sufficient data over a range of processing made to improve volumetric productivity and thus push the
TABLE 13a. Comparison of relationship between OUR and KLa for selected historical and current cultivations
OUR range KLa range
Regression Number
Scale A1 used for used for
Cultivation coefficient, of
(nominal volume) (atm) regression regression
r2 cultivations
(mmol/l-h) (mmol/l-h-atm)
Historical (1992 to mid-2001)
C. sorbophila 280 l 0.22 0.97 3053 120230 11
800 l 0.22 0.94 50105 230470 11
C. chilensis 280 l 0.46 0.99 75140 160300 4
800 l 0.32 0.99 65118 155320 3
S. cerevisiae QC2B 800 l 0.19 0.98 4092 180460 22
S. cerevisiae 1375 280 l 0.19 0.91 2566 140340 33
800 l 0.17 0.84 5367 285370 11
1900 l 0.17 0.99 5160 258308 4
E. coli RR1 280 l 0.16 0.90 3186 190500 20
1900 l 0.18 0.88 2597 151596 5
E. coli DH5 1000 l 0.17 0.99 80150 412780 16
E. coli OP50-1 1900 l 0.075 0.95 3949 177303 3
Recent (mid-2001 to 2002)
C. chilensis 280 l 0.31 0.97 71158 230535 7
1200 l 0.18 0.92 7395 296445 5
E. coli DH5 280 l 0.39 0.96 5098 250373 4
Equation 12a: OUR = A1KLa+ B1. Based on peak OUR measured during fermentation (not necessarily peak OUR capacity of equipment).
TABLE 13b. Relationship between KLa (mmol/l-h-atm) and Pg/VL (hp/1000 l) for historical and current results
Superficial Pg/VL range KLa range
Scale Regression Number
velocity, used for used for
Cultivation (nominal volume) A2 B2 coefficient, of
Vs regression regression
(impeller type) r2 cultivations
(cm/s) (hp/1000 l) (mmol/l-h-atm)
Single scale results
S. avermitilis a 800 l (R) 0.667 0.58 1.8 NA 0.678.0 3590 1
(converted to hp/1000 l 800 l (M) 0.667 0.59 2.2 NA 0.332.0 50180 1
from kw/1000 l)
A. terreus b 800 l (R) 0.51.0 0.6 1.9 NA 0.385.6 30200 1
(converted to hp/1000 l 0.8 1.2 NA 0.314.4 445 1
from kw/1000 l)
S. cerevisiae 1375 1000 l (R) 1.131.7 0.96 0.97 0.92 3.77 485897 6
E. coli RR1 1900 l (M) 0.750.84 0.96 1.6 0.81 4.114.7 150600 5
E. coli DH5 280 l (M) 2.0 0.98 1.5 0.89 8.318.9 230535 7
Multi-scale equation
Equation 9b as applied to 100 l19000 l 1.58.1 0.67 NA NA 120 NA NA
facility vessels
Equation 12b: logKLa = A2 log(Pg/VL) + B2. Range of superficial velocities assumed constant for calculated values. Common (base 10) logarithm
utilized. R, Rushton; M, Maxflo T; A, A315. NA, Calculation not applicable.
a
See Ref. 58.
b
See Ref. 23.
limits of existing and future fermentor design capacity. When c : exponent (Eq. 4)
more scale-up experience is gained over a broad range of CC : Chemineer CD-6 top/CD-6 bottom impeller con-
volumes, the utility of various scale-up methodologies can figuration
better be evaluated. Throughout these evaluations, an effec- CL : measured concentration of dissolved oxygen in
tive scale-down model is key to effective trouble shooting at broth, mmol/l or %saturation
the large scale, and its development should be a priority. Csat : concentration of dissolved oxygen in broth at sat-
uration, mmol/l or % saturation
NOMENCLATURE dCO2 : dissolved carbon dioxide
DI : diameter of impeller, m
a : exponent (Eq. 9) DO : dissolved oxygen
b : exponent (Eq. 9) DT : diameter of vessel, OD, m
A1, B1: slope and intercept constants (Eq. 12a) DTi : diameter of vessel, i, OD, m
A2, B2: slope and intercept constants (Eq. 12b) f1 : proportionality constant (Eq. 4)
A : Lightnin A315 impeller (pumping downwards) f2 : proportionality constant (Eqs. 9, 9ae)
configuration f3 : proportionality constant (Eqs. 10ag)
Fo : equivalent kill for observed sterilization tempera- m : growth rate, h1

ture relative to that at 121C, min r : density, g/cm3
gc : gravitational acceleration conversion factor, 1 kg h : viscosity, g/cm-s (poise)
m/Ns2
HE : Chemineer HE-3 top/CD-6 bottom impeller con-
figuration
REFERENCES
HL : height of liquid in tank (including bottom dish), m
HT : total height of tank (including top and bottom 1. Van Brunt, J.: Scale-up: the next hurdle. Bio/Technology, 3,
dishes), m 419423 (1985).
HTT : tangent to tangent height of tank (excluding top 2. Ju, L.-K. and Chase, G. G.: Improved scale-up strategies of
and bottom dishes), m bioreactors. Bioprocess Eng., 8, 4953 (1992).
3. Votruba, J. and Sobotka, M.: Physiological similarity and
Im : mixedness index bioreactor scale-up. Folia Microbiol., 37, 331345 (1992).
ITS : impeller tip speed, pNDI, m/s 4. Naveh, D.: Scale-up of fermentation for recombinant DNA
KLa : volumetric mass transfer coefficient, mmol/l-atm-h, products. Food Technol., 39, 102108 (1985).
or KLa/H, h1, where H is Henrys law coefficient 5. Banks, G. T.: Scale-up of fermentation processes, p. 170
(assumed to be about 1 mmol/l-atm for fermenta- 266. In Wiseman, A. (ed.), Topics in enzyme and fermenta-
tion broth) tion biotechnology, vol. 3. John Wiley & Sons, New York
M : Chemineer Maxflo T impeller (pumping down- (1979).
6. Young, T. B.: Fermentation scale-up: industrial experience
wards) configuration with a total environmental approach. Ann. N.Y. Acad. Sci.,
MC : Chemineer Maxflo T top/CD-6 bottom impeller 326, 165180 (1979).
configuration 7. Reisman, H. B.: Problems in scale-up of biotechnology pro-
N : impeller speed, rev/min (rpm) duction processes. Crit. Rev. Biotechnol., 13, 195223 (1993).
NA : flow (aeration) number, Q/NDI3 8. Jem, K. J.: Scale-down techniques for fermentation. BioPharm,
NB : number of baffles 3, 3039 (1989).
Ng : number of generations 9. Enfors, S. O., Jahic, M., Rozkov, A., Xu, B., Hecker, M.,
NI : number of impellers Jurgen, B., Kruger, E., Schweder, T., Hamer, G., OBeirne,
D., and 22 other authors: Physiological responses to mixing
Nmax : maximum impeller speed, rev/min (rpm) in large scale bioreactors. J. Biotechnol., 85, 175185 (2001).
NP : power number, external/inertial, (1/N 3DI5) (Pogc/r) 10. Ettler, P.: Scale-up and scale-down techniques for fermenta-
NRe : impeller-based Reynolds number, inertial/viscous, tions of polyene antibiotics. Collect. Czech. Chem. Commun.,
rNDI2/h 55, 17301740 (1990).
OTR : oxygen transfer rate, mmol/l-h 11. Sweere, A. P. J., Luyben, K. C. A. M., and Kossen, N. W. F.:
OUR : oxygen uptake rate, mmol/l-h Review. Regime analysis and scale-down: tools to investigate
Pg : aerated power input, watts or hp the performance of bioreactors. Enzyme Microb. Technol., 9,
386398 (1987).
Pg/VL : gassed power input per unit volume, hp/1000 l 12. Trilli, A.: Scale-up of fermentation, p. 277307. In Demain,
Po : unaerated power input, watts or hp A. L. and Solomon, N. A. (ed.), Manual of industrial microbi-
Po/VL : ungassed power input per unit volume, hp/1000 l ology and biotechnology. American Society for Microbiol-
PT : total pressure in vessel including head pressure, ogy, Washington, D.C. (1986).
kg/cm2 13. Oldshue, J. Y.: Lets understand mixing. Chemtech, 11, 554
Q : volumetric air flow rate, l/min (lpm) 561 (1981).
Qmax : maximum volumetric air flow rate, l/min (lpm) 14. Lilly, M. D.: Problems in process scale-up, p. 7989. In
Q/VL : volumetric air flow rate per unit vessel liquid vol- Nisbet, L. J. and Winstanley, D. J. (ed.), Bioactive microbial
products. Academic Press, New York (1983).
ume, 1/min (vvm) 15. Humphrey, A.: Shake flask to fermentor: what have we
R : Lightnin Rushton impeller configuration learned? Biotechnol. Prog., 14, 37 (1998).
Ro : equivalent nutrient degradation for observed ster- 16. Bylinkina, E. S. and Birukov, V. V.: The problem of scale-
ilization temperature relative to that at 121C, min up in antibiotic biosynthesis, p. 105115. In Terui, G. (ed.),
r2 : linear regression coefficient Proc. 4th Intern. Ferment. Symp., Ferment. Technol. Today.
Tmix : mixing time, s The Society of Fermentation Technology, Japan, Osaka (1972).
VL : working volume of vessel, l or m3 17. Fox, R. I.: The applicability of published scale-up criteria to
commercial fermentation processes, p. 8083. In Proc. 1st
VLi : working volume of vessel, i, l Eur. Cong. Biotechnol., part 1. Verlag Chemie, New York
Vs : superficial velocity, cm/s (1978).
VT : total (not nominal) volume of vessel, l 18. Takebe, H., Takane, N., Hiruta, O., Satoh, A., Kataoka,
VTi : total volume of vessel, i, l H., and Tanaka, H.: Scale-up of bialaphos production. J.
VFD : variable frequency drive Ferment. Bioeng., 78, 9399 (1994).
vvm : vessel volume per minute of air flow rate (Q/VL), 19. Okada, S. and Iwamatu, S.: Scale-up production of milbe-
1/min mycin by Streptomyces hygroscopicus subsp. aureolacrimo-
X : cell density, g dcw/l sus with control of internal pressure, temperature, aeration
and agitation. J. Chem. Technol. Biotechnol., 70, 179187
XN : cell number (or mass) in culture after a time inter- (1997).
val, # or g 20. Flickinger, M. C., Greenstein, M., Bremmon, C., and
XNo : initial cell number or mass in inoculum, # or g Conlin, J.: Strain selection, medium development and scale-
YX/O2 : cell yield on oxygen, g dcw/mmol/l up of toyocamycin production by Streptomyces chrestomy-
ceticus. Bioprocess Eng., 5, 143153 (1990). 43. Bylund, F., Guillard, F., Enfors, S., Tragardh, C., and
21. Byun, T.-G., Zeng, A.-P., and Deckwer, W.-D.: Reactor Larsson, G.: Scale down of recombinant protein production:
comparison and scale-up for the microaerobic production of a comparative study of scaling performance Escherichia
2,3-butanediol by Enterobacter aerogenes at constant oxygen coli fed-batch culture in laboratory scale stirred tank and
transfer rate. Bioprocess Eng., 11, 167175 (1994). aerated plug flow bioreactor. Bioprocess Eng., 20, 377389
22. Mooyman, J. G.: Scaling oxygen mass transfer in agitated (1999).
fermentors. Biotechnol. Bioeng., 29, 180186 (1987). 44. George, S., Larsson, G., Olsson, K., and Enfors, S. O.:
23. Gbewonyo, K., Hunt, G., and Buckland, B.: Interactions of Comparison of the Bakers yeast performance in laboratory
cell morphology and transport processes in the lovastatin fer- and production scale Saccharomyces cerevisiae perfor-
mentation. Bioprocess Eng., 8, 17 (1992). mance study using scale-up fermentor model. Bioprocess Eng.,
24. Junker, B. H., Stanik, M., Barna, C., Salmon, P., Paul, E., 18, 135142 (1998).
and Buckland, B. C.: Influence of impeller type on power in- 45. Schweder, T., Kruger, E., Xu, B., Jurgen, B., Blomsten, G.,
put in fermentation vessels. Bioprocess Eng., 18, 401412 Enfors, S., and Hecker, M.: Monitoring of genes that re-
(1998). spond to process-related stress in large-scale bioprocesses.
25. Junker, B. H., Mann, Z., and Hunt, G.: Retrofit of CD-6 Biotechnol. Bioeng., 65, 151159 (1999).
(Smith) impeller in fermentation vessels. Appl. Biochem. Bio- 46. Xu, B., Jahic, M., Blomsten, G., and Enfors, S.: Glucose
technol., 89, 6783 (2000). overflow metabolism and mixed acid fermentation in aerobic
26. Einsele, A.: Scaling-up bioreactors. Process Biochem., 7, 13 large scale fed-batch processes with Escherichia coli. Appl.
14 (1978). Microbiol. Biotechnol., 51, 564571 (1999).
27. Ettler, P.: Problems and possibilities in fermentation scale-up 47. Buckland, B. C.: Fermentation exhaust gas analysis using
procedure, p. 297305. In Malik, V. S. and Pradma, S. (ed.), mass spectrometry. Bio/Technology, 3, 982988 (1985).
Industrial biotechnology. Oxford and IBH, New Delhi (1992). 48. George, H. A., Powell, A. L., Dahlgren, M. E., Herber,
28. Charles, M. and Wilson, J.: Fermenter design, p. 1157 W. K., Maigetter, R. Z., Burgess, B. W., Stirdivant, S. M.,
1189. In Flickinger, M. C. and Drew, S. W. (ed.) Bioprocess and Greasham, R. L.: Physiological effects of TGFa-PE40
technology: fermentation, biocatalysis, and bioseparation, expression in recombinant Escherichia coli JM109. Biotech-
vol. 2. John Wiley and Sons, New York (1999). nol. Bioeng., 40, 437445 (1992).
29. Kossen, N. W. F. and Oosterhuis, N. M. G.: Modelling and 49. Lee, C., Sun, W. J., Burgess, B. W., Junker, B. H., Reddy,
scaling-up of bioreactors, p. 571605. In Rehm, H.-J. and J., Buckland, B. C., and Greasham, R. L.: Process optimi-
Reed., G. (ed.), and Brauer, H. (vol. ed.), Biotechnology, zation for large-scale production of TGF-a-PE40 in recombi-
vol. 2. VCG Verlagsgesellschaft, Berlin (1985). nant Escherichia coli: effect of medium composition and in-
30. Brown, D. E.: Industrial-scale operation of microbial proc- duction timing on protein expression. J. Ind. Microbiol. Bio-
esses. J. Chem. Technol. Biotechnol., 32, 3446 (1982). technol., 18, 260266 (1997).
31. Metzner, A. B. and Pigford, R. L.: Scale-up theory and its 50. Gbewonyo, K., Rohrer, S. P., Lister, L., Burgess, B., Cully,
limitations, p. 1647. In Fleming, R. (ed.), Scale-up in prac- D., and Buckland, B.: Large scale cultivation of the free liv-
tice. Reinhold Publishing Corporation, New York (1958). ing nematode Caernorhabditis elegans. Bio/Technology, 12,
32. Swartz, J. R.: Scale-up of genetically engineered products, 5154 (1994).
p. 368391. In The world biotech report 1984, vol. 2. Pinner, 51. Marshall, C. T., Lilly, M. D., Gbewonyo, K., and Buckland,
Middlesex, UK (1984). B. C.: Use of comparative reasoning tools for evaluation of
33. Bartholomew, W. H.: Scale-up of submerged fermentations. the effect of sterilization conditions on fermentations to pro-
Adv. Appl. Microbiol., 2, 289300 (1960). duce acidic fibroblast growth factor. Biotechnol. Bioeng., 47,
34. Ozbek, B. and Gayik, S.: The studies on the oxygen mass 688695 (1995).
transfer coefficient in a bioreactor. Process Biochem., 36, 52. Schulman, C. A., Ellis, R. W., and Maigetter, R. Z.: Pro-
729741 (2001). duction of hepatitis B surface antigen (PreS2 +S) by high cell
35. Buckland, B. C.: The translation of scale in fermentation proc- density cultivations of a recombinant yeast. J. Biotechnol.,
esses: the impact of computer process control. Bio/Technol- 21, 109126 (1991).
ogy, 2, 875883 (1984). 53. Zhang, J., Reddy, J., Salmon, P., Buckland, B., and
36. Benz, G. T.: Optimize power consumption in aerobic fer- Greasham, R.: Process characterization studies to facilitate
menters. CEP, 99, May, 3235 (2003). validation of a recombinant protein fermentation, p. 1227. In
37. Cooney, C. L., Wang, D. I. C., and Mateles, R. I.: Measure- Kelley, B. and Ramelmeier, A. (ed.), Validation of biophar-
ment of heat evolution and correlation with oxygen consump- maceutical manufacturing processes. ACS Symp. Ser., 698.
tion during microbial growth. Biotechnol. Bioeng., 11, 269 American Chemical Society, Washington, D.C. (1998).
281 (1968). 54. Katz, L., Marcin, C., Zitano, L., King, J., Price, K.,
38. Junker, B. H., Beshty, B., and Wilson, J.: Sterilization-in- Grinberg, N., Bhupathy, M., McNamara, J., Bergan, J.,
place of concentrated nutrient solutions. Biotechnol. Bioeng., Greasham, R., and Chartrain, M.: Screening and selection
62, 501508 (1998). of a microbial lipase for the stereospecific hydrolysis of ver-
39. Hubbard, D. W.: Scaleup strategies for bioreactors contain- lukast. J. Ind. Microbiol., 11, 8995 (1993).
ing non-Newtonian broths. Ann. N.Y. Acad. Sci., 506, 600 55. Junker, B. H., Mann, Z., Seeley, A., Zhang, J., and
607 (1987). Greasham, R.: Use of glucose feeding to produce concen-
40. Flores, E. R., Perez, F., and de la Torre, M.: Scale-up of trated yeast cells. Appl. Biochem. Biotechnol., 97, 6378
Bacillus thuringiensis fermentation based on oxygen transfer. (2002).
J. Ferment. Bioeng., 83, 561564 (1997). 56. Chartrain, M., Roberge, C., Chung, J., McNamara, J.,
41. Diaz, A. and Acevedo, F.: Scale-up strategy for bioreactors Zhao, D., Olewinski, R., Hunt, G., Salmon, P., Roush, D.,
with Newtonian and non-Newtonian broths. Bioprocess Eng., Yamasaki, S., Wang, T., Grabowski, E., Buckland, B., and
21, 2123 (1999). Greasham, R.: Asymmetric bioreduction of (2-(4-nitro-
42. Wang, D. I. C., Cooney, C. L., Demain, A. L., Dunnill, P., phenyl)-N-(2-oxo-2-pyridin-3-yl-ethyl)-acetamide) to its
Humphrey, A. E., and Lilly, M.: Fermentation and enzyme corresponding (R) alcohol [(R)-N-(2-hydroxy-2-pyridin-3-
technology, p. 194211. John Wiley and Sons, New York yl-ethyl)-2-(4-nitro-phenyl)-acetamide] by using Candida
(1979). sorbophila MY1833. Enzyme Microb. Technol., 25, 489496
(1999). of hydrofoil impellers to improve oxygen transfer efficiency

57. Chartrain, M., Greasham, R., Moore, J., Reider, P., in viscous mycelial fermentations, p. 281299. In British Hy-
Robinson, D., and Buckland, B.: Asymmetric bioreduc- drodynamics Research Association, Fluid engineering, pro-
tions: applications to the synthesis of pharmaceuticals. J. Mol. ceedings of the International Conference on Bioreactor Fluid
Catal. B: Enzym., 11, 503512 (2001). Dynamics. Cambridge, UK (1986).
58. Gbewonyo, K., DiMasi, D., and Buckland, B. C.: The use

Scale Up PDF

Uploaded by

Document Information

Original Title

Copyright

Available Formats

Share this document

Share or Embed Document

Sharing Options

Did you find this document useful?

Is this content inappropriate?

Copyright:

Available Formats

Scale Up PDF

Uploaded by

Copyright:

Available Formats

JOURNAL OF BIOSCIENCE AND BIOENGINEERING

Vol. 97, No. 6, 347364. 2004

Scale-Up Methodologies for Escherichia coli and

Received 22 August 2003/Accepted 15 March 2004

[Key words: scale-up, Escherichia coli, yeast, pilot plant, fermentor]

TABLE 1. Characteristics of laboratory and pilot scale vessels

TABLE 2. Characteristics of laboratory and pilot-plant scale impellers

TABLE 3. Geometric comparisons for laboratory and pilot scale fermentors

FIG. 2. Decline of installed, ungassed and gassed power draw per

For geometrically similar vessels in the region of turbulent

conditions from typical process development data sets. Often

Fo : equivalent kill for observed sterilization tempera- m : growth rate, h1

(1999). of hydrofoil impellers to improve oxygen transfer efficiency

You might also like