Synaptic Vesicular Localization and Exocytosis ofl-Aspartate in Excitatory Nerve Terminals: A Quantitative Immunogold Analysis in Rat Hippocampus

Gundersen, Vidar; Chaudhry, Farrukh A.; Bjaalie, Jan G.; Fonnum, Frode; Ottersen, Ole Petter; Storm‐Mathisen, Jon

doi:10.1523/jneurosci.18-16-06059.1998

Cited by 126 publications

(135 citation statements)

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“…[1][2][3][4][5][6][7]). Strongly in favour of an exocytotic release mechanism are our previous immunocytochemical results showing that K + induced depolarisation elicited depletion of L-aspartate from nerve endings, which could be inhibited by low extracellular Ca 2+ -concentrations and tetanus toxin [8][9][10]. In addition, Daspartate has been shown to be subject to exocytotic release both from cultured neurons [11] There is ample evidence that excitatory nerve endings in the brain contain functional plasma membrane excitatory amino acid transporters (EAATs) [16][17][18][19][20].…”

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confidence: 97%

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Vesicular Release of L- and D-Aspartate from Hippocampal Nerve Terminals: Immunogold Evidence~!2008-09-01~!2008-10-15~!2008-12-05~!

Holten¹,

Morland²,

Nordengen³

et al. 2008

TONEURJ

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Abstract:Glutamate is established as the most important excitatory transmitter in the brain. The transmitter status of aspartate is debated. There is evidence that aspartate is released from nerve terminals by exocytosis. However, release through excitatory amino acid transporters (EAATs) could be an alternative mechanism. We further investigated this by use of light and quantitative electron microscopic immunocytochemistry. The nerve terminal localisation of aspartate was compared to that of glutamate using antibodies specifically recognising the amino acids. Rat hippocampal slices were incubated under normal (3 mM) and depolarising (55 mM) concentrations of K + with and without the excitatory amino acid transporter inhibitor threo-beta-benzyloxyaspartate (TBOA). If aspartate is released either through reversal of the EAATs or through exchange with synaptically released glutamate, we would expect that TBOA would block the depolarisation induced release of aspartate. We found, however, that there was a substantial depletion of aspartate, as well as of glutamate, from hippocampal nerve terminals during K + induced depolarisation in the presence of TBOA. The possibility that aspartate is released through exocytosis from synaptic vesicles was further investigated by the use of a D-aspartate uptake assay, including exposure of the slices to exogenous D-aspartate and the use of D-aspartate immunogold cytochemistry to localise D-aspartate in the fixed tissue. We found that D-aspartate taken up into the terminals was concentrated in synaptic vesicles as opposed to in the cytoplasmic matrix. This is in line with the presence in synaptic vesicles of the recently identified vesicular transporter for aspartate.Keywords: Synaptic vesicles, immunocytochemistry, amino acids, electron microscopy, transport.The release of glutamate at synapses in the brain is well studied. Glutamate is released upon depolarisation of the presynaptic nerve terminal, leading to opening of voltage gated Ca 2+ channels and Ca 2+-dependent fusion of glutamate filled synaptic vesicles with the plasma membrane. The mechanism of release of L-aspartate at central synapses remains less defined. L-aspartate has been shown to be released in a Ca 2+ and clostridium toxin sensitive manner from various in vitro brain preparations (e.g. [1][2][3][4][5][6][7]). Strongly in favour of an exocytotic release mechanism are our previous immunocytochemical results showing that K + induced depolarisation elicited depletion of L-aspartate from nerve endings, which could be inhibited by low extracellular Ca 2+ -concentrations and tetanus toxin [8][9][10]. In addition, Daspartate has been shown to be subject to exocytotic release both from cultured neurons [11] There is ample evidence that excitatory nerve endings in the brain contain functional plasma membrane excitatory amino acid transporters (EAATs) [16][17][18][19][20]. The previous aspartate release data do not clearly distinguish between Laspartate release via exocytosis and via these EAATs, which could release as...

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confidence: 97%

“…Hippocampal slice experiments were performed as previously described [8,9,18]. In brief, in each experiment we…”

Section: Hippocapal Slice Incubationmentioning

confidence: 99%

Vesicular Release of L- and D-Aspartate from Hippocampal Nerve Terminals: Immunogold Evidence~!2008-09-01~!2008-10-15~!2008-12-05~!

Holten¹,

Morland²,

Nordengen³

et al. 2008

TONEURJ

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“…Aspartate immunoreactivity has been localized to synaptic vesicles of certain excitatory [10,11] and inhibitory [12] hippocampal pathways. In those pathways, aspartate immunoreactivity was associated with synaptic vesicles to the same degree as glutamate or GABA immunoreactivity.…”

Section: Introductionmentioning

confidence: 99%

“…Due to methodological differences between the two studies, however, further investigations are needed to substantiate the implied physical separation of aspartate and glutamate release sites. The colocalization of vesicular aspartate with vesicular glutamate in synaptic terminals of certain excitatory hippocampal pathways [10,11,13] and its colocalization with vesicular GABA in others [12] suggests a physiological role for aspartate different from that of other transmitter amino acids. We suggested that aspartate release at a distance from the presynaptic active zones should activate extrasynaptic NMDA receptors and that aspartate may indeed be a major endogenous agonist for these receptors [1].…”

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confidence: 99%

“…Pretreatment of neocortical synaptosomes [17], whole brain synaptosomes [6] or hippocampal slices [10,11] with Clostridial toxins inhibited chemicallyevoked aspartate release, as expected for an exocytotic process, but either a high concentration of toxin was used or the possibility of release by heteroexchange with released glutamate was not excluded. In our study of rat hippocampal synaptosomes, pretreatment with Clostridial toxins reduced glutamate release markedly, but did not reduce the simultaneous release of aspartate from the same tissue samples [1].…”

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Reduced aspartate release from rat hippocampal synaptosomes loaded with Clostridial toxin light chain by electroporation: Evidence for an exocytotic mechanism

Wang

Nadler

2007

Neuroscience Letters

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Aspartate can be released from certain hippocampal pathways along with glutamate or GABA. Although aspartate immunoreactivity has been localized to synaptic vesicles and aspartate release is Ca 2+ -dependent, there has been no clear evidence favoring an exocytotic mechanism. In particular, pretreatment with Clostridial toxins has not consistently inhibited aspartate release, even when release of glutamate from the same tissue samples was markedly inhibited. To address this issue directly, rat hippocampal synaptosomes were permeabilized transiently by electroporation in the presence of active or inactivated Clostridial toxin light chains. Loading rat hippocampal synaptosomes with the active light chain of tetanus toxin or of botulinum neurotoxins A, B or C reduced the K + -evoked release of aspartate at least as much as that of glutamate. These results confirm that aspartate is released by exocytosis in rat hippocampus. KeywordsAspartate; Excitatory amino acids; Transmitter release; Hippocampus; Exocytosis; Clostridial toxins Although hippocampal preparations have long been known to release aspartate along with the recognized transmitters glutamate and GABA [18,19], the mechanism and physiological significance of aspartate release remain unclear. Aspartate immunoreactivity has been localized to synaptic vesicles of certain excitatory [10,11] and inhibitory [12] hippocampal pathways. In those pathways, aspartate immunoreactivity was associated with synaptic vesicles to the same degree as glutamate or GABA immunoreactivity. Aspartate is coreleased with glutamate from the Schaffer collateral-commissural and dentate gyrus associationalcommissural pathways in a Ca 2+ -dependent manner [2,3,19] and could serve as a co-transmitter through its selective activation of NMDA receptors [4,22]. However, the mechanism of aspartate release appears to differ in some respects from that of the recognized amino acid transmitters. In our previous study of rat hippocampal synaptosomes, aspartate release was more sensitive than glutamate release to increases in intracellular [Ca 2+ ] outside the presynaptic active zones, was reduced by KB-R7943, an inhibitor of Na + /Ca 2+ exchange, was much less sensitive than glutamate release to block of P/Q-type voltage-dependent Ca 2+ channels, and resisted both bafilomycin A 1 , an inhibitor of vacuolar H + -ATPase, and Clostridial toxins [1].Address correspondence to J. Victor Nadler, Department of Pharmacology and Cancer Biology, Box 3813, Duke University Medical Center, Durham, NC 27710, USA. Telephone: (919) 684-5317; FAX: (919) 681-8609; E-mail: nadle002@acpub.duke.edu.. Publisher's Disclaimer: This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final citable form. Please note that during the production process errors may be discovered which could af...

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Immunocytochemical localization of neurokinin B in the rat spinal dorsal horn and its association with substance P and GABA: An electron microscopic study

2000

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Synaptic Vesicular Localization and Exocytosis ofl-Aspartate in Excitatory Nerve Terminals: A Quantitative Immunogold Analysis in Rat Hippocampus

Cited by 126 publications

References 51 publications

Vesicular Release of L- and D-Aspartate from Hippocampal Nerve Terminals: Immunogold Evidence~!2008-09-01~!2008-10-15~!2008-12-05~!

Vesicular Release of L- and D-Aspartate from Hippocampal Nerve Terminals: Immunogold Evidence~!2008-09-01~!2008-10-15~!2008-12-05~!

Reduced aspartate release from rat hippocampal synaptosomes loaded with Clostridial toxin light chain by electroporation: Evidence for an exocytotic mechanism

Immunocytochemical localization of neurokinin B in the rat spinal dorsal horn and its association with substance P and GABA: An electron microscopic study

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