Scribd Logo
Upload

Welcome to Scribd!

  • Folwchart NGS

    Uploaded by

    กรวรินทร์ ชำนาญกุล
    11 views3 pages

    Copyright

    © © All Rights Reserved

    Available Formats

    PDF, TXT or read online from Scribd

    Did you find this document useful?

    Is this content inappropriate?

    Report this Document

    Copyright:

    © All Rights Reserved
    Download as PDF, TXT or read online from Scribd
    Flag for inappropriate content
    11 views3 pages

    Folwchart NGS

    Uploaded by

    กรวรินทร์ ชำนาญกุล

    Copyright:

    © All Rights Reserved
    Download as PDF, TXT or read online from Scribd
    Flag for inappropriate content
    of 3

    Flowchart NGS Illumina, short read 500

    bp, akw per too cycle


    Erne

    Prepare Genomic DNA sample Attach DNA to Surface


    Bridge Amplification Fragment Become dsDNA

    was n e template 15s nucleotide increa


    nadapters DNA 118:
    .::
    22 3 enzyme
    7 >
    DNA

    in
    s
    template is ouregner wo rodwide

    ezemegiawiis
    i
    was DNA
    cellultrasonic -
    -
    is Uncletide
    ligase Adopters 2 Ens_Mochanic shearing
    iner vortex

    Snea,812
    -
    flow cell channels an double stranded bridge
    RE, POR
    fragmentationsel solid phase sub (flow cell)

    Image FirstBase Determine First Bese Complete Amplification Denature the Double-stranded
    misantri was laser or lied: ·a
    sequencing easie < emplify DNA inerie
    S
    denature is DNA eider
    ??
    cluster bids 1181 labeled reversible terminators, ↓Cluster Quisa
    es
    detectinsign d
    primers 118: DNA
    polymerese
    V

    Determine Second Base


    Image Second Datz
    Chemistry Cycle Sequencing over
    multiple Align
    for labeled reversible terminators, misanni were laser amaraw:, chemistry cycles VENIENTOW sos, di
    primers 118: DNA
    polymerese ·ridone and awnin Sequencing cycle dinin identified
    sor: segeneral base

    paired and
    250,250 bp deer re autput awsiered
    single end to divers

    165 -

    metagenomic sequencing library Preparation

    Analyze Prokoryotic
    16S rRNA 1,800bp

    Work flow sun

    1. Implicon primer 46bp esis overhung adapter Cillumine


    vs, 44 and
    party (
    4 Yaw PCR, adapters as: dust-index barcodes
    2.
    amplify us &

    3. Sequence on
    Miseg-Ming paired scalp no:
    Miseg us
    vergent65-hour run can
    reads, 96 indexed

    100k/semple
    4.
    Analyze MSR/BusaSpose is Missy reporter

    163 V3 and 24
    Amplicon work flow
    forward
    overhang specific
    adopter primer e
    I
    y undex (
    >
    Normalize, Sequence
    reverse DNA o

    atuch
    sy adapters
    Jag Nexters*XT Index Kit

    Amplicon primer

    7.5 klindwoth Eve s. addlaus-specific 3. 2, recommends insertcoverlop 50


    bpl
    specific sy sq/Illumina overhang b. Th 60- 65'

    16
    Amplican PCR sdepter fur, w a deselting purification in paler is write

    ferward/reverse
    primer
    mark flow
    765 libung preprintion

    Pre deni

    Amplicon PUR
    -
    denst
    sundown, aL
    product verity size
    PCR

    consumableProcedure printernal eyeare


    o vs/v4 primer Amplican PCR -550bp
    C extentio
    mix,

    PCR Clean-Up purify 163 V3/V4 on free primer/primer dimer

    Ci5w

    AMPureXP, centrifug YUM 25a) ample, Vartex AMPure 30s VM soch >
    mix 10 ass
    AMPune Nw tips seal
    plate
    Wounds DCR plate min
    1 I MIDI plate We
    dure? ricons column Iwiudes
    Ihr PCR plate
    2 min

    stand
    magnetic
    not sol
    etchremove aperitant a
    magnetic,
    Fuss
    <

    a magnet sand 2nd of H 2,200 at 80% dOH We stand 2 min is da min


    E <

    sir-dry to min 2,200 ih b. N 30s/risaries supersistentto


    b. U2 30 S C. ca supernatanti
    2 remove
    supernatent
    d. Pso remove excess ofPH

    fromear
    Amplican PCR,
    12525uh(omytrispoennam magnetzmin, carefully
    remove War Two min, a

    consin magnetstrand superintent scampernatant]


    POR platePus
    an index at
    OCR/ligation, were simple
    index 18

    Index PCR odeptors NextarexIndux Kit


    Amplicon PCR product
    indeste,
    Pastit Times
    jel-96 well an
    <asPR
    primer product a

    2. Indexe white caps (clear) A -


    H

    Index, wrong, yellow) 1-12


    -> Sarise Microser's' dwinds, min - Thermal cycles

    PCR clean-up 2

    al VertexAmPure aL AmPure index plate


    centrifuge So PCR product ->
    Edd 86

    Index plate, min to MIDI plate Index


    an 30S


    2nd etch magnet, times
    isthe
    sofefol a
    remove
    -
    oc a mix 10

    wood in her zoom der sos


    mpernetest uperment seal shake a mill

    per remove efcht remove


    superintent
    Di MIDI like 2 m

    ir-dry nomin -

    add
    remove
    te ->
    mix is time evermine marmagnzmine transfer coal supernate
    27.5dThs pHs, 5
    l
    -> 1950 library DNA

    Library penst& Misey Im


    lording laser cluster

    tube
    1.7m) microcent
    96'd, remove Misey reagent, is bucket, water both is ice in waters

    temp
    in
    stock rear

    as arecome
    -denist DNA

    in
    slatedinvent most phixcontel-Vortex, mine emise
    mine

    2.2 NOOH 8 uL

    - dilute Denot DNA

    dilute insimons ->


    mix to dent/diluter an ice

    denst & dilute Phix Control

    dilute
    ahem, routeterrain, enterthan pi phix
    1. w Phixto 4 nM dent20
    t nM Phix cue,
    +10 mM TrispH

    pascution
    8.53 a
    mix

    on root mix

    Combine Amplican &


    Phil Conte

    phixrulemix andrhertegent that black time interbate min


    5
    ->

    in

    You might also like