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皮层谷氨酸能和γ-氨基丁酸能轴突终末中突触结合蛋白、突触囊泡蛋白2和Rab3表达的分析

Analysis of Synaptotagmin, SV2, and Rab3 Expression in Cortical Glutamatergic and GABAergic Axon Terminals.

作者信息

Bragina Luca, Fattorini Giorgia, Giovedí Silvia, Melone Marcello, Bosco Federica, Benfenati Fabio, Conti Fiorenzo

机构信息

Section of Neuroscience and Cell Biology, Department of Experimental and Clinical Medicine, Università Politecnica delle Marche Ancona, Italy.

出版信息

Front Cell Neurosci. 2012 Jan 10;5:32. doi: 10.3389/fncel.2011.00032. eCollection 2011.

Abstract

We investigated whether cortical glutamatergic and GABAergic release machineries can be differentiated on the basis of the nature and amount of proteins they express, by performing a quantitative analysis of the degree of co-localization of synaptotagmin (SYT) 1 and 2, synaptic vesicle protein 2 (SV2) A and B, and Rab3a and c in VGLUT1+, VGLUT2+, and VGAT+ terminals and synaptic vesicles (SVs) in rat cerebral cortex. Co-localization studies showed that VGLUT1 puncta had high levels of SV2A and B and of Rab3c, intermediate levels of SYT1, and low levels of SYT2 and Rab3c; VGLUT2 puncta exhibited intermediate levels of all presynaptic proteins studied; whereas vesicular GABA transporter (VGAT) puncta had high levels of SV2A and SYT2, intermediate levels of SYT1, Rab3a, and Rab3c, and low levels of SV2B. Since SV2B is reportedly expressed by glutamatergic neurons and we observed SV2B expression in VGAT puncta, we performed electron microscopic studies and found SV2B positive axon terminals forming symmetric synapses. Immunoisolation studies showed that the expression levels of the protein isoforms varied in the three populations of SVs. Expression of SYT1 was highest in VGLUT1-SVs, while SYT2 expression was similar in the three SV groups. Expression of SV2A was similarly high in all three SV populations, except for SV2B levels that were very low in VGAT SVs. Finally, Rab3a levels were similar in the three SV groups, while Rab3c levels were highest in VGLUT1-SVs. These quantitative results extend our previous studies on the differential expression of presynaptic proteins involved in neurotransmitter release in GABAergic and glutamatergic terminals and indicate that heterogeneity of the respective release machineries can be generated by the differential complement of SV proteins involved in distinct stages of the release process.

摘要

我们通过对大鼠大脑皮层中VGLUT1+、VGLUT2+和VGAT+终末及突触小泡(SVs)中突触结合蛋白(SYT)1和2、突触小泡蛋白2(SV2)A和B以及Rab3a和c的共定位程度进行定量分析,研究了皮质谷氨酸能和γ-氨基丁酸能释放机制是否可以根据它们所表达蛋白质的性质和数量来区分。共定位研究表明,VGLUT1斑点具有高水平的SV2A和B以及Rab3c,SYT1水平中等,SYT2和Rab3a水平低;VGLUT2斑点在所研究的所有突触前蛋白中表现出中等水平;而囊泡γ-氨基丁酸转运体(VGAT)斑点具有高水平的SV2A和SYT2,SYT1、Rab3a和Rab3c水平中等,SV2B水平低。由于据报道SV2B由谷氨酸能神经元表达,且我们在VGAT斑点中观察到了SV2B的表达,因此我们进行了电子显微镜研究,发现SV2B阳性轴突终末形成对称突触。免疫分离研究表明,三种突触小泡群体中蛋白质异构体的表达水平各不相同。SYT1在VGLUT1-SVs中的表达最高,而SYT2在三个突触小泡组中的表达相似。除了VGAT突触小泡中SV2B水平非常低外,SV2A在所有三个突触小泡群体中的表达同样很高。最后,Rab3a水平在三个突触小泡组中相似,而Rab3c水平在VGLUT1-SVs中最高。这些定量结果扩展了我们之前关于参与GABA能和谷氨酸能终末神经递质释放的突触前蛋白差异表达的研究,并表明各自释放机制的异质性可由参与释放过程不同阶段的突触小泡蛋白的差异互补产生。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/c6d8/3254050/f2ad7e6fcc51/fncel-05-00032-g001.jpg

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