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In this study we provide
In this study we provide biochemical and immunohistochemical evidence for the localization of the glycine transporter GLYT1 in synaptic vesicles. Previously, it was thought that GLYT1 was exclusively a glial protein (Zafra et al., 1995a). However, due to a partial discrepancy between mRNA and protein distribution (Smith et al., 1992, Zafra et al., 1995b), additional immunohistochemical studies were carried out and these revealed the existence of neuronal forms of GLYT1. The neuronal GLYT1 is mainly located in terminals of glutamatergic nature since they also contain a vesicular glutamate transporter, either vGLUT1 or vGLUT2 (Cubelos et al., 2005). In the present report, a careful analysis of the subcellular GLYT1 distribution in the mossy fiber terminals of the stratum lucidum of the hippocampus, accesible to confocal microscope analysis due to their large size, suggests that GLYT1 is localized not only in the Bleomycin Sulfate membrane but also in the intracellular compartment. Consistent with this possibility, previous immunogold EM data revealed the presence of GLYT1 in intracellular locations, especially in the flanking region of the presynaptic active zones (Cubelos et al., 2005). In agreement with this observation, biochemical data presented in this report support the presence of GLYT1 in the microsomal fraction derived from lysed synaptosomes. Moreover, further purification of the microsomal fraction through a sucrose density gradient to obtain highly purified synaptic vesicles shows that GLYT1 is modestly enriched in the vesicular fraction, at a difference with the plasma membrane marker Na+/K+-ATPase that is depleted. Furthermore, the direct immunoisolation of a purified fraction of synaptic vesicles, using immobilized anti-synaptophysin antibodies, strongly supports the localization of GLYT1 in these synaptic vesicles. The localization of GLYT1 in vesicles containing synaptophysin was confirmed by immunogold EM. GLYT1 was found in about 40% of the purified vesicles and more than 90% of the GLYT1 labelled vesicles also contained synaptophysin. Although this is an unusual localization for a Na+ and Cl− dependent neurotransmitter transporter, this is a property shared by the two closer relatives of the family: GLYT2 (Nuñez et al., 2009) and the proline transporter PROT (Renick et al., 1999). This localization contrasts with that of the GABA transporter GAT1 that was found in small vesicles, similar to synaptic vesicles in flotation characteristics but lacking the synaptic vesicle marker synaptophysin (Deken et al., 2003). A vesicular localization has been also observed for the choline transporter, although this transporter belongs to a different gene family (Ferguson et al., 2003). This localization might couple the release of neurotransmitter with its reuptake, a possibility that seems plausible for the choline transporter in cholinergic terminals and perhaps for GLYT2 in glycinergic ones, since these terminals release acetylcholine and glycine, respectively, upon neuronal depolarization. Arrival of these transporters to the plasma membrane during the depolarization-induced vesicle fusion would increase the capability for removal neurotransmitter from the synaptic cleft just after the massive release of neurotransmitter. This might be also the case for GLYT1. Recent observations indicate that glycine is released from glutamatergic terminals in hippocampal neurons upon depolarization (Muller et al., 2013). Moreover, release of glycine from hippocampal and cortical slices and synaptosomes has been reported. This release contains both calcium dependent and calcium-independent components (Russo et al., 1993, Galli et al., 1993, Luccini et al., 2008). However, an important question remains to be answered: assuming a vesicular release of glycine through the calcium-dependent mechanism, how is glycine accumulated into synaptic vesicles? Since glutamatergic terminals do not contain VIAAT, the vesicular transporter for glycine and GABA that is present in inhibitory neurons, several other possibilities can be considered. First, it might exist a novel and yet unidentified vesicular transporter for glycine. Second, the vesicular transporter for glutamate might allow the entrance of glycine, similarly to the recent observation of GABA entering the vesicles through the vesicular monoamine transporter vMAT2 (Tritsch et al., 2012). Third, GLYT1 itself might mediate the accumulation of glycine into the synaptic vesicles either by equilibration of cytoplasmic and lumenal concentrations of glycine or, even, by some type of uncharacterized active transport within the vesicles. Due to the topology of GLYT1, the entrance of glycine within the vesicles would be equivalent to efflux through the plasma membrane. Whether the intracellular ambient might provide the necessary conditions for this hypothetical mechanism remains to be determined.