GABA Receptors and The Immune System-012012
GABA Receptors and The Immune System-012012
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Contents
Abstract ............................................................................................................................................. 3
PART 1. THE GABA SYSTEM ............................................................................................................... 3
GABA synthesis and transport ...................................................................................................... 3
GABAA receptors ........................................................................................................................... 5
Structure................................................................................................................................... 5
Function and distribution ......................................................................................................... 6
GABAB receptors ........................................................................................................................... 8
Structure and signaling ............................................................................................................ 8
Distribution ............................................................................................................................ 10
GABA and the immune system ....................................................................................................... 11
Cells of the immune system ....................................................................................................... 11
GABA metabolism and the immune system............................................................................... 12
GABAA receptors and the immune system ................................................................................. 13
GABAB receptors and the immune system ................................................................................. 14
GABA, GABA receptors and the immune system in vivo ............................................................ 16
PART 2. MINI INTERNSHIP............................................................................................................... 17
Materials and methods .............................................................................................................. 17
Results ........................................................................................................................................ 17
Discussion ................................................................................................................................... 18
References ...................................................................................................................................... 20
Acknowledgements
I would like to thank dr. P.A.J. Henricks at the Division of Pharmacology, Utrecht Institute for
Pharmaceutical Sciences, Faculty of Science, Utrecht University, for providing the facilities for my
experimental work and general supervision. Also thanks to S. de Kivit for extensive supervision of the
experiments.
Cover page picture: Electron microscopic image of a single human lymphocyte. National Cancer Institute USA
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Abstract
Traditionally known as purely an inhibitory neurotransmitter, -aminobutyric acid (GABA), its
receptors and enzymes involved in GABA metabolism and catabolism have been shown to be widely
distributed outside the brain and central nervous system. One of the organ systems expressing
GABAA and GABAB receptors and other parts of the GABA system is the immune system. GABA and
GABA analogous have primarily an inhibitory effect on the immune system, although the effect of
activating GABAB receptors seems to be more complex and include immune stimulation. Molecular
changes evoked by GABAergic compounds also translate to potential in vivo treatment of diseases
associated with the immune system. Activation of immune cells leads in some cases to increased
GABAB receptor expression, suggesting a natural function of these receptors in immune system
functioning.
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any important extent in vivo due to the co-localisation of high activity of succinic semialdehyde
dehydrogenase (SSADH) and GABA-T [8]. In the brain, GABA-T is primarily expressed in glial and
endothelial cells [7]. Therefor, it can be concluded that (in the CNS) GABA anabolism and catabolism
occur in the neurons and glial cells, respectively. Although an integral part of GABAergic systems in
the CNS, GABA-T is also expressed in a variety of other tissues, including liver, pancreas, kidneys,
lungs, heart, stomach, hair follicles, the placenta and even platelets [8,10]. On a sub-cellular level
expression seems to be concentrated to the inner mitochondrial membrane [8].
-Ketoglutarate
Glutamate
GABA-T
GAD
Succinic semialdehyde
SSADH
-Aminobutyric acid
Succinic acid
Figure 1. GABA shunt: synthesis and degradation. The neurotransmitter GABA is synthesized
by GAD from glutamate, which is converted from -ketoglutarate, an intermediate of the Krebs
cycle, by GABA-T. GABA can be degraded by GABA-T to succinic semialdehyde and subsequently
to succinic acid, also an intermediate in the Krebs cycle. -aminobutyric acid; GABA-T, -
aminobutyric acid transaminase; GAD, glutamic acid decarboxylase; SSADH, succinic
semialdehyde dehydrogenase.
After release into the synaptic cleft, GABA is rapidly removed from the intercellular space by
specific transporters to prevent GABA spillover to neighboring synapses and tonic activation of GABA
receptors [11]. The majority of the released GABA is transported back into the synapse, while a
smaller fraction is taken up by astrocytes surrounding the synapse [12]. Currently, four of these
GABA transporters (GATs) have been described: GAT-1 through GAT-3 (rat nomenclature) and the
Betain/GABA transporter type 1 (BGT-1), a receptor that uses both GABA and betain as substrates.
GATs are GABA Na+/Cl- coupled transporters, with the Na+ gradient being the primary driving force
for GABA uptake, while Cl- can significantly enhance uptake [10]. GAT-1 seems to be conserved in
mammals displaying a high degree of amino acid sequence homology in rat, mouse and human and
essentially identical pharmacological properties. GAT-2 and GAT-3 show a higher degree of sequence
identity with each other and BGT-1 than with GAT-1. In the adult rat brain GATs are mainly localized
in astrocytes and some neuronal terminals, hypothesized to be GABAergic synapses. Expression of
GAT-1 differs strongly between brain regions, with high expression in the forebrain, intermediate
expression in the cerebellum and lower expression in the majority of the hindbrain [13].
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GABAA receptors
In the brain, 17-20% of all neurons are GABAergic and most of the physiological activities of
GABA are generated through GABAA receptors (GABAA-Rs) [14]. These ionotropic receptors or ligand-
gated ion channel (LGIC) are chloride anion (Cl-) channels that can be opened and activated by the
endogenous neurotransmitter GABA and several drug classes, including benzodiazepines,
barbiturates, steroids, anesthetics and convulsants. As the primary receptor for GABA in the CNS,
GABAA receptors are involved in a variety of behavioral and cognitive processes [14].
Structure
GABAA receptors are composed of 5 protein subunits, which all have a large extracellular N-
terminal domain, four transmembrane (TM) domains, a large intracellular loop between TM3 and
TM4 and a relatively short C-terminal domain (figure 2A). The number of different subunits is 19, not
including different splice variants, and that makes this set the largest of any among the mammalian
ion channel receptors [14]. These subunits can be divided into 2 categories: 16 (1-6, 1-3, 1-3, , ,
and ) which can be combined to form the traditional GABAA-R and 3 (rho) subunits (Greek
letters signify >70% sequence identity). Receptors containing subunits are sometimes referred to as
GABAC receptors, though that is recommended against by the International Union of Basic and
Clinical Pharmacology (IUPHAR) [15]. The most prevalent GABAA-Rs contain , and subunits, but
native receptors lacking a subunit do exist. In the CNS approximately 75-80% of the receptors
contain 2, while 1 and 3 are rarer. The most common subunit is 1, often colocalized with 2
and 2. Among the subunits 2 is the most abundant, while 1 is the least common *15+.
Interestingly, birds express also 4 and 4 subunits, but seems to lack both and subunits *16+.
The protein subunits are combined in different ways and arranged around a central pore,
which allows Cl- to pass through (figure 2B). The receptors roughly share their structure with other
N
C
ys
C
ys
C
TM1
TM2
TM3
TM4
AA B B
Cl-
Figure 2. GABAA receptor and subunit structure. A) Each subunit consists of a large N-terminal
domain, 4 transmembrane domains (TMs), a large loop between TM 3 and 4 and a relatively short C-
terminal domain. The characteristic cys-loop is located in the N-terminal domain. B) Five subunits are
grouped around a central pore to form a GABAA receptor.
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closely related Cys-loop pentameric LGICs. This superfamily also includes nicotinic acetylcholine
receptors (nAChR), inhibitory glycine receptors, ionotropic 5-HT3 (serotonin) receptors and a Zn2+-
activated ion channel [16]. All 44 subunit members of the superfamily show around 30% sequence
homology and greater secondary and tertiary structure similarity [15]. They all use similar sequences
and functional domains in ion channel structure, endogenous ligand binding sites and membrane
topology. In 2005 the structure of the nAChR in a species of electric ray (Torpedo marmorata) was
resolved to a resolution of 4 , through cryo-electron microscopy and image reconstruction [17].
More recently the structure of a toxin-bound murine nAChR-subunit was determined in 2007 [18].
Also two high resolution X-ray studies of prokaryotic pentameric LGICs have provided significant
insight into structure [19,20]. And, although the structure of the GABAA-R has not been determined,
it can therefore be approximated through homology modeling. The resulting models of the majority
of GABAA receptors (those containing 1 , 2 and 2 subunits), show not only the arrangement of
subunits within the receptor, but also several structural features in the extracellular domain and their
binding pockets [15]. The benzodiazepine binding site (Bz BS) is located at the interface of an and -
subunit. Classic benzodiazepines, such as diazepam, exhibit a high affinity for specific subunit
combinations. These diazepam sensitive (DS) receptors include those composed of 12, 22,
32 and 52, as well as less well known analogues containing the 3-subunit. Some Bz BS
ligands are also able to interact with receptors composed of 42 and 62, while diazepam is not.
These can therefore be referred to as diazepam insensitive (DI) receptors [21].
The combination of specific subunit combinations and distinct effects allows the development of
subtype selective ligands in order to elicit a specific respons [21]. Also other non- subunits can be
important in neuropharmacology: 2-subunits are involved in anxiety, while -subunits have a role in
learning and memory [22]. Akinci and Schofield provide a comprehensive summary on receptor
subunits and associated effects [23]. Although the 5 subunit is relatively rare in the brain, its
expression is high in the hippocampus, which corresponds with its link to temporal and spatial
memory. The 4 and 6 subunits are highly expressed in the forebrain and cerebellum *15+.
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Outside of the mammalian CNS and peripheral nervous sytem (PNS), GABAA receptor subunits
are also expressed in a variety of other tissues. In cell lines subunits are also expressed. For example,
mRNA for the 2, 3, 2, 3, 2 and subunits can be found in the NCI-H295R adrenocortical
carcinoma cell line, which could be sufficient to form functional receptors [24]. In mice TM3 Leydig
cells, mRNA of subunits 1, 2 1, 3 and 1 was present and cell proliferation was significantly
increased by selective GABAA receptor agonists [25]. In an article on experiments in rats, Akinci and
Schofield report mRNA detection of many GABAA-R subunits in a number of peripheral tissues [23].
Placenta, ovaries and testis all have a large repertoire of subunits, while the repertoires of the small
intestine and uterus are smaller. Interestingly, in the endocrine tissues in these experiments, 3
mRNA was only present in the testis. In the testis, mRNA of 1-5, 1-3, 1 and 2, , , 1 and 2 was
also reported, while in the uterus 1, 2 and 6, 3, 1, and 1 mRNA was detected [23]. GABAA-Rs
are also present in other parts of the female reproductive system such as the oviduct mucosa and
fallopian tubes [26].
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GABAB receptors
In addition to acting on the ionotropic GABAA receptor, GABA is also an endogenous agonist of
the GABAB receptor (GABAB-R). The GABAB-R is a member of the large metabotropic G-protein
coupled receptor (GPCR) superfamily, with 367 known members in humans as of 2003, a major
target of pharmaceutical drugs and involved in for example taste, smell, metabolism, reproduction,
development, hormonal homeostasis, and behavior [33]. It can be found in the brain, at both
excitatory and inhibitory synapses, and in several other organs. By interacting with multiple
downstream signaling cascades, GABAB-Rs have many physiological roles [34].
GABA
GABAB1 GABAB2
1 2 3 4 5 6 7
G-protein
C
Figure 3. General GABAB receptor heterodimer structure. The functional GABAB receptor is
composed of the 2 subunits and associates with heterotrimeric G proteins upon GABA binding.
8
As a type of GPCR, GABAB-Rs transduce extracellular signals via heterotrimeric G proteins,
particularly the Gi- and Go-types. Through binding and activating G protein subunits, GABAB-Rs are
coupled to a variety of effectors, including enzymes and ion channels. For example, GABAB-Rs couple
to several types of voltage-gated Ca2+ channels. High-voltage activated Ca2+ channels of the N- or
P/Q-type or intermediate-voltage-activated R-type can be potently inhibited by G complexes, that
bind specific channel subunits upon activation and liberation from Go proteins [39,40]. L-type Ca2+
channels (Long-Lasting) can be both inhibited and augmented by GABAB-R activation. The latter
effect may be partly mediated by protein kinase A (PKA) or, more effectively, protein kinase C (PKC)
activity [41]. More recently, it has also been reported that the GABAB2 subunit can interact directly
with L-type Ca2+ channels. Through the formation of a protein complex, this interaction modulates
Ca2+ influx [42]. In addition to Ca2+ channels, GABAB-Rs are also coupled to K+ channels. Kir3 (or GIRK)
is a subfamily of inwardly rectifying potassium channels. Activation of Kir3 channels results in situ in
a K+ efflux, thereby hyperpolarizing the cell and inhibiting excitability [39]. It is likely GABAB-Rs are
also coupled to other types of K+ channels. Specifically blocking rapidly inactivating A-type K+
channels, for example, inhibits a GABAB agonist-induced current in neurons [39]. Small-conductance
Ca2+-activated K+ (SK) channels, important in regulating synaptic plasticity, memory and learning, are
activated by GABA [43]. This activation may be due to inhibition of cyclic adenosine monophosphate
(cAMP) production through GABAB-Rs [39].
Another signaling pathway induced by GABAB-Rs is the PI-3-kinaseAkt pathway [47]. Akt, also
known as protein kinase B (PKB), regulates key cellular functions, such as nutrient metabolism, cell
growth, apoptosis and survival by several mechanisms, including inactivating the pro-apoptotic
proteins Bad and caspase-9 [48]. Activation of GABAB-Rs, for example, leads to neuroprotection via
PI-3-kinase, independent of cAMP levels [49]. The PI-3-kinase binds the activated GPCR, which actives
it to convert membrane-bound PI(4,5)P2 to PI(3,4,5)P3. The PIP3 recruits the two kinases Akt and
phosphoinositidine-dependent protein kinase 1 (PDK1) and the latter activates Akt in conjunction
with a third kinase. The activated Akt dissociates from PIP3 and phosphorylates target proteins [50].
Interestingly, activation of Akt by GABAB-Rs may also be direct, since GABAB2 subunits can interact
and complex with Akt [47].
Also an important target of GABAB-Rs is the protein kinase C (PKC) family, which shares a
significant sequence homology with PKB [50,51]. The PKC family has 12 members in mammals and
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other eukaryotes. All PKC isoforms share a highly conserved carboxy-terminal kinase domain [52].
Analogous to other GPCRs coupled to Gi- and Go-type G proteins, when G complexes are
released following G protein activation by the GABAB-R, they are able to activate the phospholipase
C (PLC) [51]. Subsequently, activation of PLC leads to the formation of diacylglycerol (DAG) and
inositol 1,4,5-triphosphate (IP3). The latter product acts as an agonist on IP3-gated Ca2+ channels,
opening them to release Ca2+ into the cytosol from stores in the endoplasmatic reticulum (ER).
Combined, the free Ca2+ and DAG recruit PKC to the plasma membrane and activate it. An important
downstream of PKC is nuclear factor kappa-light-chain-enhancer of activated B cells (NF-B), a
transcription factor which regulates genes involved in cell growth and differentiation and
inflammatory response. Another target of PKC is the protein kinase D (PKD) family, which can also be
activated by DAG *53+. Its likely, that pathway allows GABAB-Rs to activate ERK, a mitogen-activated
protein kinase (MAPK) also involved in proliferation and differentiation and a downstream target of
several growth factor receptors [54,55].
Distribution
Like GABAA receptors and other parts of the GABA system, GABAB-Rs are expressed in a wide
range of tissues and organs. In the CNS, GABAB-Rs are expressed in the thalamus, cerebellum,
hippocampus, cerebral cortex, dentate gyrus, interpenduncular nucleus and dorsal root ganglia
[56,57]. GABAB-Rs can also be found in peripheral organs, such as the esophagus. In rats, GABBR1 is
present in the adrenals, pituitary, spleen, kidney, liver and prostate [57]. Functional receptors have
also been reported in airway epithelial cells and smooth muscle, islets of Langerhans, the placenta
and fallopian tubes [55,58]. Expression of GABAB1a, GABAB1e (a truncated subunit) and GABAB2 has
been detected in the NCI-H295R adrenocortical carcinoma cell line [24]. Interestingly, GABAB-Rs are
also expressed in cancer cells. In human prostate cancer cells, the GABAB-R agonist baclofen
promotes migration, while suppression has also been reported, for example in hepatocellular
carcinoma cells [59].
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GABA and the immune system
The components of the immune system can be categorized in various ways, one of which is the
distinction between humoral and cellular immunity. The former focuses primarily on antibodies,
but the complement system and other antimicrobial substances may also be categorized as part of
the humoral immune system. The cellular immune system includes a diverse repertoire of cell types
and is extensively intertwined with the humoral part.
Figure 4. Basic hematopoiesis in humans. Hematopoietic Stem Cells (HSCs) in the bone marrow
give rise to all lymphoid and myeloid lineages.
Lymphoid progenitor
Natural Killer cell
HSC
Basophil
T lymphocyte
Eosinophil
B lymphocyte
Myeloid progenitor
Neutrophil
Dendritic cell
Macrophage
Monocyte
Erythrocyte Thrombocytes
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and eliminate virus-infected and cancer cells. Sun and Lanier recently provided valuable insight in NK
cell development and function [61].
Cells considered part of the adaptive immunity consist of T and B lymphocytes. The latter are the
producers of all classes of antibodies, also known as immunoglobulins. Some antibodies are
produced in response to infection, while IgM, for example, is also secreted naturally by B cells *62+.
T lymphocytes can be further divided into a number of types, which include CD8+ (cytotoxic) T cells,
which can be activated by CD4+ T (helper) cells. Zhang and Bevan recently reviewed CD8+ T cell
activation and functioning [63]. Other types include Regulatory T (Treg) cells, which can suppress
immune activation, and more recently discovered and not completely understood T cells and
Natural killer T (NKT) cells. Turchinovich and Pennington [64] summarize current research on T
cells, while Godfrey and Rossjohn have published a review on NKT cells [65].
GABA has been reported in cultured resting murine macrophages, and was also found in
extract of macrophages cultured from peripheral blood monocytes [68]. Macrophages and
lymphocytes in skin of psoriasis patients are positive for GABA [69]. The enzyme GAD65 was present
in significant amounts in dendritic cells (DCs) and in lower concentrations also in peritoneal
macrophages, suggesting these cells posses functional synthetic machinery to produce GABA [70].
Macrophages, DCs and T lymphocytes also secrete GABA. Stimulation of macrophages and DCs with
lipopolysaccharide (LPS) increased GAD65 expression, while the amount of secreted GABA wasnt
influenced significantly. Stimulation of CD4+ T cells with anti-CD3 and anti-CD28 antibodies also had
no effect on the concentration of GABA in the medium. The presence of GABA-T was reported in
macrophages and T lymphocytes. Stimulation increased the expression of GABA-T in T cells, but did
not significantly alter expression in macrophages [70]. Expression of GAD67 mRNA was reported in
70-80% of resting and 100% of activated lymphocytes [71]. Both B cells and T cells were present in
this lymphocyte isolate. It is likely, that the studied population was mainly formed by T cells since a
specific T lymphocyte mitogen (phytohemagglutinin; PHA) was used for stimulation and the T:B cell
ratio was about 3:1,. B-T cell interactions however, may have influenced expression. The vesicular
inhibitory amino acid transporter (VIAAT) protein, detected in most resting and activated isolated
lymphocytes, was clustered, suggesting this transporter of GABA and glycine may be associated with
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vesicular compartments that store GABA in these cells. GAT-1 mRNA was present in 50% of resting
lymphocyte samples, while in activated samples, both GAT-1 and GAT-2 mRNA expression was
reported. Stimulated lymphocytes showed significantly higher GABA uptake than resting cells.
Depletion of Na+ largely diminished this increase [71]. Intact GAD65 and GAD67 are also present in
neutrophil granulocytes, indicating neutrophils may also produce GABA [47]. Surprisingly, neither
GAD65 nor GAD67 are expressed by microglia, resident macrophages of the CNS, but these cells do
express GABA-T [72].
Table 2. GABAA receptor subunits expression by mammalian immune cells
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monocytes were researched [77]. Of all the 19 known subunits, only 2 mRNA was present in freshly
prepared monocytes, while THP-1 cells also expressed 4, 1 and subunits.
Although several types of immune cells do express GABAA receptor subunit mRNA and protein, it
can not be deduced from that, that these cells also posses fully functional receptors. Bath et al.
studied the effects of GABAA-R ligands on cytokine production and intracellular signaling [70]. The
anti-convulsant topiramate, a drug with GABAA-R agonist properties, inhibited the cytokine
production of antigen challenged murine splenocytes in dose-dependent manner. Both pro-
inflammatory tumor necrosis factor (TNF), interleukin 17 (IL-17) and IL-6 and anti-inflammatory IL-10
showed significant reduced production. Activated purified T lymphocytes on the other hand, showed
no significant influence of GABAA-R agonists on proliferation and production of interferon (IFN),
TNF, IL-17 or IL-6. Surprisingly, Tian et al. did report inhibition of antigen-induced T cell proliferation
by the GABAA-R agonist muscimol [78]. Peritoneal macrophages isolated from mice treated with
either the GABA-T inhibitor vigabatrin or topiramate, produced after LPS stimulation significantly
lower quantities of pro-inflammatory IL-1 [70]. The same diminished production was also seen in
dendritic cells. Interestingly, macrophages from animals treated with topiramate reduced the
production of pro-inflammatory IFN by T cells when co-cultured. The reverse of this setting did not
have a comparable effect. Production of other cytokines by macrophages was also modified by
GABAA-R activation [76]. GABA added to cultured murine peritoneal macrophages decreased IL-6 and
IL-12 production, while the non-competitive GABAA-R antagonist picrotoxin, reversed this inhibition
in a dose-dependent manner, suggesting the effect was mediated by GABAA-Rs.
Functional research on GABAB receptors and the immune system is relatively scarce compared to
GABAA receptors. Pretreating neutrophils with 10 M of the GABAB-R agonist baclofen significantly
induced chemotaxis, measured as migration across a polyethylene membrane, although less effective
than chemoattractant fMLP (N-Formylmethionine leucyl-phenylalanine) [47]. Furthermore, the
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GABAB-R antagonist CGP52432 significantly inhibited baclofen-stimulated neutrophil chemotaxis.
Reduction of chemotaxis by the reversible PI-3-K inhibitor LY294002 was partly reverted by baclofen,
suggesting induction of chemotaxis in neutrophils is mediated by PI-3 kinase. Functional GABAB-Rs
expressed by PBMCs were also reported to have a notable effect on cytokine production [82]. PBMCs
activated with PHA showed a significant 40% decrease in TNF and a slight (non-significant) increase
in IL-4 production in response to baclofen, while IFN, IL-2, IL-5, IL-6 and IL-10 showed no significant
changes. Microglia stimulated with LPS secreted a significant amount of pro-inflammatory IL-6 and IL-
12p40 compared to controls [81]. Co-incubation of LPS and baclofen caused a considerable
concentration-dependent reduction in secretion of these cytokines. Baclofen had no notable effect
on IL-6 and IL-12 in unstimulated controls. Migration of CD133+ HSPCs is primarily regulated by
stromal cell-derived factor-1 (SDF-1) [80]. Adding SDF-1 increase locomotion of these cells by
approximately 50% and co-incubation with baclofen normalizes migration. Treatment with baclofen
alone results in a slight decrease of migration compared to untreated controls. The reduction by this
GABAB-R agonist is comparable to GABA itself in the same concentration, indicating the effect is
primarily mediated by GABAB-Rs. In addition to mentioned molecular effects, GABAB-R agonists
potentially influence various other cellular functions (figure 5).
Ligand
GABAB receptor
Ca2+ channel
PIP2
PIP3 AC
PI3K
PLC
PDK1 kinase
ATP
cAMP
PKC
Akt/PKB
Ca2+ PKA
Bad
Caspase-9
PKD
Cytochrome C
P47phox NF-B
Erk1/2
TNFR CBP Pol II
TLRs CREB
TCR
corticosteroids
Gene expression
Growth factors
COX2 Cytokines
Chemokines NUCLEUS
CYTOPLASM
Figure 5. Important signaling pathways associated with the GABAB receptor and the immune
system. AC, Adenylate cyclase; Bad, Bcl-2-associated15 death promoter; COX2, cyclooxygenase-2;
Erk1/2, Extracellular signal-regulated kinase 1/2; TCR, T cell receptor; TLR, Toll-like receptor; TNFR,
tumor necrosis factor receptor
GABA, GABA receptors and the immune system in vivo
The influence of GABAA and GABAB-R agonists and other GABAergic agents on cytokine
production and cellular signaling results in various in vivo effects. Treatment of mice with
experimental autoimmune encephalomyelitis (EAE), a model used to mimic inflammatory
demyelinating diseases of the CNS such as multiple sclerosis, with GABA-T inhibitor vigabatrin or anti-
convulsant topiramate significantly reduces the severity of symptoms [70]. Non-obese diabetic (NOD)
mice are prone to developing autoimmune insulin dependent diabetes mellitus. Splenic T cells
respond spontaneously to cell antigens by secreting the pro-inflammatory cytokine IFN [75].
Adding GABA inhibits this spontaneous response ex vivo. Consequently, NOD/scid (severe combined
immunodeficiency) mice implanted with pallets releasing GABA over a period of 21 or 60 days,
showed a much slower progression to diabetes. NOD mice implanted two times consecutively with a
similar pallet, releasing GABA over a total period of 180 days, showed a similar effect. While placebo
treated controls developed diabetes from 20 weeks of age on, the GABA treated group showed no
diabetes prevalence until after 40 weeks. Collagen-induced arthritis (CIA) is a mouse model sharing
many immunological and pathological features with human rheumatoid arthritis. Mice treated orally
with GABA had a lower disease severity than controls [83]. Splenic T lymphocytes in vivo primed with
bovine collagen type II (bCII) peptide showed reduced proliferation ex vivo in a GABA-containing
medium. Levels of total immunoglobulin G (IgG) and subtype IgG2a specific for bCII in serum of
collagen immunized mice, were lower in those treated with GABA. Mice suffering from allergic
contact dermatitis benefited of treatment with GABAB-R agonist baclofen [82]. The ear swelling
response for example, was markedly reduced by intraperitoneal baclofen injection. Histology also
showed a reduction of inflammatory infiltrate, visible as a reduced number of macrophages,
monocytes, CD45+ lymphocytes and neutrophils. A study on the GABAB-R agonist phenibut
demonstrated the immunomodulating effects in immune hyperactivation [84]. Mice injected with
Pseudomonas aeruginosa-derived LPS showed characteristics of immune stress, including increased
delayed-type hypersensitivity and phagocytic activity of neutrophils. These parameters normalized
after phenibut intra-abdominal injection. In contrast to these immunosuppressive effects, another
study on phenibut showed it to be a potent immunostimulant [85]. Mice intraperitoneally injected
with the immunosuppressant cyclophosphamide had a reduced spleen weight, thymus weight,
delayed-type hypersensitivity response, antibody response and reduced numbers of nucleated cells
in the spleen and thymus. Treatment with different phenibut salts normalized one or more of these
parameters.
The mentioned in vivo and in vitro research both point to the potential of modifying the
peripheral GABA system in the clinic. Pharmaceuticals that inhibit GABA degradation could be used
to reduce inflammation in autoimmune diseases. GABAA receptor agonists could serve the same
purpose, especially when designed to hinder activation in the CNS. Both local (topical) and systemic
use is possible. GABAA-R antagonists and compounds which reduce GABA synthesis may be useful in
treating drug-induced immune suppression, for example in patients treated with cytostatics. GABAB
receptor agonists, especially those recently designed to act primarily on peripheral receptors [86],
have potential in treating autoimmune disease. Its potential seems more restricted, but may be
successful in diseases dominated by TNF-, such as rheumatoid arthritis, asthma and inflammatory
bowel disease [87-89].
16
PART 2. MINI INTERNSHIP
Results
Using forward scatter (FSC) and GABBR2 FITC fluorescence, it can be determined that human
blood contains several mononuclear cell populations, some of which are weakly or strongly express
GABAB2 receptors (figure 6). To further identify the different cell types present and the extent of their
GABBR2 expression, samples were labeled for CD4, a surface marker primarily expressed by T helper
lymphocytes and monocyte/macrophage-marker CD14. In addition, cells were stimulated with either
LPS or anti-CD3/28 to explore the effect of activation on GABBR2 expression.
Most of unstimulated CD14+ monocytes expressed GABAB2 receptors on their membranes (figure
7B, red). Also a number of CD14- cells expressed GABAB2 receptors. Interestingly, after stimulation of
the PBMCs with LPS, the number of cells expressing membrane GABAB2 receptors increased in both
CD14+ (figure 7C, red) and CD14- cells. Stimulation of unfractionated PBMCs with anti-CD3 and anti-
CD28 antibodies seems to have increased membrane-bound CD14 and slightly increased both CD14
and GABBR2 expressing cells (figure 8A, blue). Surprisingly, co-stimulation with both anti-CD3 and
17
+
Figure 7. GABAB2 receptor expression by monocyte CD14 cells. Based on FSC and SSC monocyte
populations were selected (A, P2 green) and CD14 expression was plotted against GABBR2 unstimulated (B)
and LPS-stimulated (C).
anti-CD28 antibodies in addition to LPS ameliorated the increase in CD14+GABBR2+ cell caused by LPS
(resp. figures 8B, blue and 7C, red).
Based on cell size and complexity, the cell cluster most likely to contain CD4+ T cells was gated
(figure 9A, red). As shown in figure 9B, this cluster includes both CD4+ (upper quadrants), which are
most likely T helper cells, and CD4- cells, which include other lymphocytes such as B cells, CD8+ T cells
and NK cells. Large numbers of CD4- lymphocytes expressed GABAB2 receptors (figure 9B, green),
while practically no GABBR2+CD4+ lymphocytes were present (figure 9B, purple). Stimulation with LPS
did not significantly alter the number of GABBR2+ lymphocytes (figure 9C). Incubation of the PBMCs
with anti-CD3 and anti-CD28 antibodies did also not notably influence GABBR2 expressing numbers
(figure 9D). Not surprisingly, stimulation with both antibodies and LPS did not increase the number of
GABBR2+ cells (figure 9E).
Discussion
Although not as pronounced as GABAA receptors, GABAB receptors do have immunomodulatory
effects [82]. Analogous to several other neurotransmitter receptors [86], including GABAA receptor
subunits, membrane GABAB2 levels are influenced by T cell and monocyte stimulation. It is highly
likely that immune cells expressing GABBR2 also express GABBR1, as functional GABAB receptors
have been identified on several immune cell types (page 14). Direct activation of monocytes with LPS
18
Figure 9. GABBR2 expression
on lymphocytes. Based on
FSC and SSC the cell
population most likely to contain
+
CD4 T cells and other small
lymphocytes was selected (A)
+
and membrane CD4
expression was plotted against
GABBR2 in unstimulated gated
cells (B), LPS (C), anti-CD3/28
(D) and anti-CD3/28 + LPS
stimulated selected PBMCs (E).
led to an increase of membrane GABBR2 expressing monocytes. Specific T cell stimulation did also
increase the number of GABBR2+ monocytes and slightly increased the amount of GABBR2
expression on monocytes. This indicates GABBR2 expression in monocytes can be induced via T cells.
As GABAB-R agonists have anti-inflammatory properties [82], this increased receptor expression may
possibly temper monocyte activation and proliferation in vivo. Treatment with both antibodies and
LPS does not increase or induce GABBR2 expression in monocytes. These effects may be mediated by
cell-cell contact or cytokines, as cytokine production in response to anti-CD3/28 and LPS differs
slightly and may compensate for or complement each other. Treatment with different cytokines can
elucidate the specific mechanism. None of the activation strategies induced GABBR2 expression in T
lymphocytes, suggesting functional GABAB-Rs may not have any significant function in T cell
activation and proliferation.
Activation of monocytes and T lymphocytes with both anti-CD3/28 and LPS did not modify
GABBR2 expression on monocytes. Anti-CD3 and anti-CD28 antibodies mimic T cell receptor (TCR)
binding to an antigen presented in a major histocompatibility complex (MHC), combined with a
costimulatory signal. LPS mimics the presence of gram-negative bacteria. Since treatment with the
antibodies and LPS did not influence GABBR2 expression on monocytes, while treatment with either
separately did, it stands to reason that in vivo immune activation by both peptide antigens and non-
peptide microbial products also does not influence GABBR2 expression on monocytes. This allows
immune activation to proceed in the presence of both types of foreign substances, while immune
activation is reduced or blocked by peripheral GABA when only one type is present.
19
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