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Action Ach in Causing Vasodilation
Action Ach in Causing Vasodilation
History
o Acetylcholine (ACh) was first identified in the year 1914 by Henry Hallett Dale for
its actions on heart tissue. It was confirmed as a neurotransmitter by Otto Loewi,
who initially gave it the name Vagusstoff because it was released from the vagus
nerve. Both received the 1936 Nobel Prize in Physiology or Medicine for their
work. Acetylcholine was also the first neurotransmitter to be identified.
Chemistry
Function
o Acetylcholine has functions both in the peripheral nervous system (PNS) and in
the central nervous system (CNS) as a neuromodulator.
o In the central nervous system, acetylcholine and the associated neurons form a
neurotransmitter system, the cholinergic system, which tends to cause anti-
excitatory actions
*The author acknowledges the contribution of the previous authors of this chapter, George
Thomas, PhD, & Peter Ramwell, PhD.
Discovery of Endogenously Generated Nitric Oxide
The first indication that NO is generated in cells came from studies of cultured macrophages,
which showed that treatment with inflammatory mediators, such as bacterial endotoxin,
resulted in the release of nitrate and nitrite, molecules that can form from the breakdown of
NO. Similarly, injection of endotoxin in animals elevated urinary nitrite and nitrate.
The second indication came from studies of vascular regulation. Several molecules, such as
acetylcholine, were known to cause relaxation of blood vessels. This effect occurred only when
the vessels were prepared so that the luminal endothelial cells covering the smooth muscle of
the vessel wall were retained. Subsequent studies showed that endothelial cells respond to
these vasorelaxants by releasing a soluble endothelial-derived relaxing factor (EDRF). EDRF
acts on vascular muscle to elicit relaxation. These findings prompted an intense search for the
identity of EDRF.
Exogenous application of NO or organic nitrates, which are metabolized to NO, were known to
elicit a variety of cellular effects including inhibition of platelet aggregation and vasorelaxation.
The cellular effects of NO were particularly intriguing, since they appeared to induce the
activation of highly specific physiologic responses, rather than more general cytotoxic
responses. Comparison of the biochemical and pharmacological properties of EDRF and NO led
to the conclusion that NO is the major bioactive component of EDRF. These findings made it
clear that exogenously applied NO and NO-releasing compounds (nitrates, nitrites,
nitroprusside; see Chapters 11 and 12) elicited their effects by recruiting physiologic signaling
pathways that respond to endogenously generated NO. NO was subsequently found to be
synthesized and have signaling roles in other tissues in addition to endothelial cells, notably
neurons, immune system cells, and skeletal muscle.
Nitric Oxide Synthesis, Signaling Mechanisms, & Inactivation
Synthesis
NO, written as NO· to indicate an unpaired electron in its chemical structure, or simply NO, is a
highly reactive signaling molecule that is made by one or more of three closely related NO
synthase (NOS, EC 1.14.13.49) isoenzymes, each of which is encoded by a separate gene and
named for the initial cell type from which it was isolated (Table 19–1). These enzymes, neuronal
NOS (nNOS or NOS-1), macrophage or inducible NOS (iNOS or NOS-2), and endothelial NOS
(eNOS or NOS-3), despite their names, are each expressed in a wide variety of cell types, often
with an overlapping distribution. These isoforms generate NO from the amino acid L -arginine in
an O2- and NADPH-dependent reaction (Figure 19–1). This enzymatic reaction involves
enzyme-bound cofactors, including heme, tetrahydrobiopterin, and flavin adenine dinucleotide
(FAD). In the case of nNOS and eNOS, NO synthesis is triggered by agents and processes that
increase cytosolic calcium concentrations. Cytosolic calcium forms complexes with calmodulin,
an abundant calcium-binding protein, which then binds and activates eNOS and nNOS. On the
other hand, iNOS is not regulated by calcium, but is constitutively active. In macrophages and
several other cell types, inflammatory mediators induce the transcriptional activation of the iNOS
gene, resulting in accumulation of iNOS and generation of increased quantities of NO.
Table 19–1 Properties of the Three Isoforms of Nitric Oxide Synthase (NOS).
Property Isoform Names
NOS-1 NOS-2 NOS-3
Other names nNOS (neuronal NOS) iNOS (inducible NOS) eNOS (endothelial NOS)
Chromosome 12 17 7
Figure 19–1
Synthesis and reactions of nitric oxide (NO). L-NMMA inhibits nitric oxide synthase. NO
complexes with the iron in hemoproteins (eg, guanylyl cyclase), resulting in the activation of
cGMP synthesis and cGMP target proteins such as protein kinase G. Under conditions of
oxidative stress, NO can react with superoxide to nitrate tyrosine.
Signaling Mechanisms
NO mediates its effects by covalent modification of proteins. There are three major effector
targets of NO (Figure 19–1):
Metalloproteins
NO interacts with metals, especially iron in heme. The major target of NO is soluble guanylyl
cyclase (sGC), an enzyme that generates cyclic GMP from guanosine triphosphate (GTP). sGC
contains heme, which readily binds NO, resulting in enzyme activation and elevation in
intracellular cGMP levels. cGMP activates protein kinase G (PKG), which phosphorylates
specific proteins. In blood vessels, NO-dependent elevations in cGMP and PKG activity result in
the phosphorylation of proteins that lead to reduced cytosolic calcium levels and subsequently
reduced contraction of vascular smooth muscle. NO also has cytotoxic effects when synthesized
in large quantities, eg, by activated macrophages. For example, NO inhibits metalloproteins
involved in cellular respiration, such as the citric acid cycle enzyme aconitase and the electron
transport chain protein cytochrome oxidase. Inhibition of the heme-containing cytochrome P450
enzymes by NO is a major pathogenic mechanism in inflammatory liver disease.
Thiols
NO reacts with thiols (compounds containing the –SH group) to form nitrosothiols. In proteins,
the thiol moiety is found in the amino acid cysteine. Upon exposure to NO, certain proteins are
found to accumulate nitrosothiols, which can activate or inhibit the activity of these proteins.
This post-translational modification, termed S-nitrosylation or S-nitrosation, requires either
metals or oxygen to catalyze the formation of the nitrosothiol adduct. Indeed, NO undergoes both
oxidative and reductive reactions, resulting in the formation of a variety of oxides of nitrogen
that can nitrosylate thiols, nitrate tyrosines (below), or which are stable oxidation products
(Table 19–2). Although the physiologic roles of protein nitrosylation are not fully established,
major targets of S-nitrosylation are H-ras, a regulator of cell proliferation that is activated by S-
nitrosylation, and the metabolic enzyme glyceraldehyde-3-phosphate dehydrogenase, which is
inhibited when it is S-nitrosylated. Denitrosylation of proteins is poorly understood but may
involve enzymes, such as thioredoxin, or chemical reduction by intracellular reducing agents.
Glutathione, a major intracellular sulfhydryl-containing compound, can also be S-nitrosylated
under physiologic conditions to generate S-nitrosoglutathione. Nitrosoglutathione may serve as
an endogenous long-lived adduct or carrier of NO. Vascular glutathione is decreased in diabetes
mellitus and atherosclerosis, and the resulting deficiency of S-nitrosoglutathione may account for
the increased incidence of cardiovascular complications in these conditions.
Name Structure Known Function
Nitric oxide (NO) N=O Vasodilator, platelet inhibitor, immune regulator,
neurotransmitter
Nitroxyl anion (NO–) N–=O Can form from nonspecific donation of an electron from
metals to NO
Tyrosine Nitration
NO reacts very efficiently with superoxide to form peroxynitrite (ONOO–), a highly reactive
oxidant that leads to DNA damage, nitration of tyrosine, and oxidation of cysteine to disulfides
or to various sulfur oxides (SOx). Several cellular enzymes synthesize superoxide, and the
activity of these enzymes, as well as NO synthesis, is increased in numerous inflammatory and
degenerative diseases, resulting in an increase in peroxynitrite levels. Numerous proteins have
been found to be susceptible to peroxynitrite-catalyzed tyrosine nitration, and this irreversible
modification can be associated with either activation or inhibition of protein function. The
presence of tyrosine nitration in tissue correlates with tissue damage, although a direct causal
role of tyrosine nitration in the pathogenesis of any disease has not been definitively established.
Protein tyrosine nitration is also used as a marker for the presence of oxidative and nitrosative
stress. Peroxynitrite-mediated protein modification is regulated by intracellular levels of
glutathione, which can protect against tissue damage by scavenging peroxynitrite. Factors that
regulate the biosynthesis and decomposition of glutathione may have important consequences on
the toxicity of NO.
Inactivation
The lability of NO is related to its rapid reactions with metals and reactive oxygen species. Thus,
NO reacts with heme and hemoproteins, including oxyhemoglobin, which catalyze NO oxidation
to nitrate. NO reactions with hemoglobin may also result in partial S-nitrosylation of
hemoglobin, resulting in transport of NO throughout the vasculature. NO is also inactivated by
superoxide, and scavengers of superoxide anion such as superoxide dismutase may protect NO,
enhancing its potency and prolonging its duration of action.
Pharmacologic Manipulation of Nitric Oxide
The primary strategy to reduce NO generation in cells is to use NOS inhibitors. The majority of
these inhibitors are arginine analogs that bind to the NOS arginine-binding site. Since each of the
NOS isoforms has high sequence similarity, most of these inhibitors do not exhibit selectivity for
any of the NOS isoforms. In inflammatory disorders and sepsis (see below), inhibition of the
iNOS isoform is potentially beneficial, whereas in neurodegenerative conditions, nNOS-specific
inhibitors are needed. However, administration of nonselective NOS inhibitors leads to
concurrent inhibition of eNOS, which impairs its homeostatic signaling and also results in
vasoconstriction and potential ischemic damage. Thus, newer NOS isoform-selective inhibitors
are being designed that exploit subtle differences in substrate binding sites between the isoforms,
as well as newer inhibitors that prevent NOS dimerization, the conformation required for
enzymatic activity. The efficacy of NOS isoform-selective inhibitors in medical conditions is
under investigation.
NO donors, which release NO or related NO species, are used to elicit smooth muscle relaxation.
Different classes of NO donors have differing biologic properties, related to the nature of the NO
species that is released and the mechanism that relates to their release.
Organic Nitrates
Organic Nitrites
Organic nitrites, such as the volatile antianginal amyl nitrite, also require metabolic activation to
elicit vasorelaxation, although the responsible enzyme has not been identified. Nitrites are
arterial vasodilators and do not exhibit the rapid tolerance seen with nitrates.
Sodium Nitroprusside
Sodium nitroprusside, which is used for rapid pressure reduction in arterial hypertension,
generates NO in response to light as well as chemical or enzymatic mechanisms in cell
membranes. See Chapter 11 for additional details.
No Gas Inhalation
Alternate Strategies
Vascular Effects
NO has a significant effect on vascular smooth muscle tone and blood pressure. Numerous
endothelium-dependent vasodilators, such as acetylcholine and bradykinin, act by increasing
intracellular calcium levels, which induces NO synthesis (Figure 19–2). Mice with a knockout
mutation in the eNOS gene display increased vascular tone and elevated mean arterial pressure,
indicating that eNOS is a fundamental regulator of blood pressure. The effects of vasopressor
drugs are increased by inhibition of NOS.
Figure 19–2
Regulation of vasorelaxation by endothelial-derived nitric oxide (NO). Endogenous
vasodilators, eg, acetylcholine and bradykinin, activate NO synthesis in the luminal endothelial
cells, leading to calcium (Ca2+) efflux from the endoplasmic reticulum into the cytoplasm.
Calcium binds to calmodulin (CaM), which activates endothelial NO synthase (eNOS),
resulting in NO synthesis from L-arginine. NO diffuses into smooth muscle cells, where it
activates soluble guanylyl cyclase and cGMP synthesis from guanosine triphosphate (GTP).
cGMP binds and activates protein kinase G (PKG), resulting in an overall reduction in calcium
influx, and inhibition of calcium-dependent muscle contraction. PKG can also block other
pathways that lead to muscle contraction. cGMP signaling is terminated by phosphodiesterases,
which convert cGMP to guanosine monophosphate (GMP).
Apart from being a vasodilator, NO protects against thrombosis and atherogenesis through
several mechanisms. A major mechanism involves the inhibition of proliferation and migration
of vascular smooth muscle. In animal models, myointimal proliferation following angioplasty
can be blocked by NO donors, by NOS gene transfer, and by NO inhalation.
NO also reduces endothelial adhesion of monocytes and leukocytes, key features of the early
development of atheromatous plaques. This effect is due to the inhibitory effect of NO on the
expression of adhesion molecules on the endothelial surface. In addition, NO may act as an
antioxidant, blocking the oxidation of low-density lipoproteins and thus preventing or reducing
the formation of foam cells in the vascular wall. Plaque formation is also affected by NO-
dependent reduction in endothelial cell permeability to lipoproteins. The importance of eNOS in
cardiovascular disease is supported by experiments showing increased atherosclerosis in animals
deficient in eNOS by pharmacologic inhibition. Atherosclerosis risk factors, such as smoking,
hyperlipidemia, diabetes, and hypertension, are associated with decreased endothelial NO
production, and thus enhance atherogenesis.
Septic Shock
Sepsis is a systemic inflammatory response caused by infection. Endotoxin components from the
bacterial wall along with endogenously generated tumor necrosis factor- and other cytokines
induce synthesis of iNOS in macrophages, neutrophils, and T cells, as well as hepatocytes,
smooth muscle cells, endothelial cells, and fibroblasts. This widespread generation of NO results
in exaggerated hypotension, shock, and, in some cases, death. This hypotension is reversed by
NOS inhibitors in humans as well as in animal models (Table 19–3). A similar reversal of
hypotension is produced by compounds that prevent the action of NO (such as the sGC inhibitor
methylene blue), as well as by scavengers of NO (eg, hemoglobin). Furthermore, knockout mice
lacking a functional iNOS gene are more resistant to endotoxin than wild-type mice. However,
thus far there has been no correlation between the hemodynamic effects of relatively
nonselective NOS inhibitors and survival rate in gram-negative sepsis in humans. The absence of
benefit may reflect the inability of the NOS inhibitors to differentiate between NOS isoforms or
may reflect concurrent inhibition of beneficial aspects of iNOS signaling.
Inhibitor Mechanism Comment
N -Monomethyl-L- Competitive inhibitor, binds arginine-binding Nonselective NOS
arginine (L-NMMA) site in NOS inhibitor
Hemoglobin NO scavenger
The host response to infection or injury involves the recruitment of leukocytes and the release of
inflammatory mediators, such as tumor necrosis factor and interleukin-1. This leads to induction
of iNOS in leukocytes, fibroblasts, and other cell types, resulting in enhanced levels of NO. NO,
along with peroxynitrite that forms from its interaction with superoxide, is an important
microbicide and may have significant roles in tissue adapting to inflammatory states. Recent
studies have shown that NO stimulates the synthesis of inflammatory prostaglandins by
activating cyclooxygenase isoenzyme 2 (COX-2). In addition, NO generated during
inflammation is involved in the vasodilation, vascular permeability, and subsequent edema
associated with acute inflammation. However, in both acute and chronic inflammatory
conditions, prolonged or excessive NO production may exacerbate tissue injury. Excessive NO
production has a detrimental effect in chronic models of arthritis; dietary L-arginine
supplementation exacerbates arthritis, whereas protection is seen with iNOS inhibitors. Synovial
fluid from patients with arthritis contains increased oxidation products of NO, particularly
peroxynitrite. Psoriasis lesions, airway epithelium in asthma, and inflammatory bowel lesions in
humans all demonstrate elevated levels of NO and iNOS. Thus, inhibition of the NO pathway
may have a beneficial effect on a variety of acute and chronic inflammatory diseases.
However, NO also appears to play an important protective role in the body via immune cell
function. When challenged with foreign antigens, TH 1 cells (see Chapter 55) respond by
synthesizing NO. Inhibition of NOS and knockout of the iNOS gene can markedly impair the
protective response to injected parasites in animal models.
NO has a major role in the central nervous system as a neurotransmitter. Unlike classic
transmitters such as glutamate or dopamine, which are stored in synaptic vesicles and released in
the synaptic cleft upon vesicle fusion, NO is not stored, but synthesized on demand and
immediately diffuses to neighboring cells. NO synthesis is induced at postsynaptic sites in
neurons, most commonly upon activation of the NMDA subtype of glutamate receptor, which
results in calcium influx and activation of nNOS. In several neuronal subtypes, eNOS is also
present and activated by neurotransmitter pathways that lead to calcium influx. NO synthesized
postsynaptically may function as a retrograde messenger and diffuse to the presynaptic terminal
to enhance the efficiency of neurotransmitter release through a cGMP or S-nitrosylation-
dependent mechanism. It has been suggested that a major role for NO is in the regulation of
synaptic plasticity, the process of synapse strengthening that underlies learning and memory.
The Peripheral Nervous System
Respiratory Disorders
Nitric Oxide
Subclass Mechanism Effects Clinical Pharmacokinetics,
of Action Applications Toxicity,
Interactions
Nitric oxide (NO)
Preparations Available
References
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Napoli C, Ignarro LJ: Nitric oxide-releasing drugs. Annu Rev Pharmacol Toxicol 2003;43:97. [PMID:
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Articles in pubmed
Feng Q, Hedner T.
Ignarro LJ.
Abstract
1. Endothelial cells of blood vessels generate factors which can modulate underlying smooth
muscle tone, inducing vasorelaxation, (endothelium-derived relaxing factor, EDRF, and
endothelium-derived hyperpolarizing factor) and/or vasoconstriction (endothelium-derived
contracting factors, EDCFs, including the peptide endothelin). 2. EDRF is nitric oxide (NO) or a
RNO compound from which this oxide is released. Its half-life is very short (6-50 sec), and it
produces rapid vasodilations and inhibits platelet aggregation. 3. NO is formed from the terminal
guanidino of L-arginine, but not of D-arginine. NO effects and NO formation are inhibited by
NG-monomethyl-L-arginine (L-NMMA), but not by D-NMMA. These inhibitory effects are
blocked by L-arginine. 4. Removal of endothelium or pathological situations that can induce
endothelial dysfunction (atherosclerosis, diabetes, hypertension or subarachnoid hemorrhage)
cause increases on the vascular contractility elicited by agonists (noradrenaline, serotonin,
EDCFs, etc.). These findings suggest that EDRF produces a physiological inhibitory modulation
of vascular smooth muscle tone and its alteration produces or facilitates the development of
diseases such as hypertension or coronary and cerebral vasospasm.