Laboratory of Membrane Transport, Department of Molecular Cell Biology, University of Leuven, Leuven, Belgium.
PLoS One. 2007 May 30;2(5):e474. doi: 10.1371/journal.pone.0000474.
The mammalian CLC protein family comprises nine members (ClC-1 to -7 and ClC-Ka, -Kb) that function either as plasma membrane chloride channels or as intracellular chloride/proton antiporters, and that sustain a broad spectrum of cellular processes, such as membrane excitability, transepithelial transport, endocytosis and lysosomal degradation. In this study we focus on human ClC-6, which is structurally most related to the late endosomal/lysomal ClC-7.
Using a polyclonal affinity-purified antibody directed against a unique epitope in the ClC-6 COOH-terminal tail, we show that human ClC-6, when transfected in COS-1 cells, is N-glycosylated in a region that is evolutionary poorly conserved between mammalian CLC proteins and that is located between the predicted helices K and M. Three asparagine residues (N410, N422 and N432) have been defined by mutagenesis as acceptor sites for N-glycosylation, but only two of the three sites seem to be simultaneously N-glycosylated. In a differentiated human neuroblastoma cell line (SH-SY5Y), endogenous ClC-6 colocalizes with LAMP-1, a late endosomal/lysosomal marker, but not with early/recycling endosomal markers such as EEA-1 and transferrin receptor. In contrast, when transiently expressed in COS-1 or HeLa cells, human ClC-6 mainly overlaps with markers for early/recycling endosomes (transferrin receptor, EEA-1, Rab5, Rab4) and not with late endosomal/lysosomal markers (LAMP-1, Rab7). Analogously, overexpression of human ClC-6 in SH-SY5Y cells also leads to an early/recycling endosomal localization of the exogenously expressed ClC-6 protein. Finally, in transiently transfected COS-1 cells, ClC-6 copurifies with detergent-resistant membrane fractions, suggesting its partitioning in lipid rafts. Mutating a juxtamembrane string of basic amino acids (amino acids 71-75: KKGRR) disturbs the association with detergent-resistant membrane fractions and also affects the segregation of ClC-6 and ClC-7 when cotransfected in COS-1 cells.
We conclude that human ClC-6 is an endosomal glycoprotein that partitions in detergent resistant lipid domains. The differential sorting of endogenous (late endosomal) versus overexpressed (early and recycling endosomal) ClC-6 is reminiscent of that of other late endosomal/lysosomal membrane proteins (e.g. LIMP II), and is consistent with a rate-limiting sorting step for ClC-6 between early endosomes and its final destination in late endosomes.
哺乳动物 CLC 蛋白家族由九个成员组成(ClC-1 到 -7 和 ClC-Ka、-Kb),它们要么作为质膜氯离子通道,要么作为细胞内氯离子/质子反向转运体发挥作用,并维持着广泛的细胞过程,如膜兴奋性、跨上皮运输、内吞作用和溶酶体降解。在这项研究中,我们专注于人类 ClC-6,它在结构上与晚期内体/溶酶体 ClC-7 最为相关。
使用针对 ClC-6 COOH 末端尾部独特表位的多克隆亲和纯化抗体,我们表明,当在 COS-1 细胞中转染时,人类 ClC-6 在进化上哺乳动物 CLC 蛋白之间保守性差的区域被 N-糖基化,该区域位于预测的螺旋 K 和 M 之间。三个天冬酰胺残基(N410、N422 和 N432)已通过突变确定为 N-糖基化的接受位点,但似乎只有两个位点同时被 N-糖基化。在分化的人神经母细胞瘤细胞系(SH-SY5Y)中,内源性 ClC-6 与晚期内体/溶酶体标志物 LAMP-1 共定位,但与早期/再循环内体标志物如 EEA-1 和转铁蛋白受体不共定位。相比之下,当在 COS-1 或 HeLa 细胞中瞬时表达时,人类 ClC-6 主要与早期/再循环内体标志物(转铁蛋白受体、EEA-1、Rab5、Rab4)重叠,而不与晚期内体/溶酶体标志物(LAMP-1、Rab7)重叠。类似地,在 SH-SY5Y 细胞中转染过量的人类 ClC-6 也导致外源性表达的 ClC-6 蛋白在早期/再循环内体中定位。最后,在瞬时转染的 COS-1 细胞中,ClC-6 与去污剂抗性膜部分共纯化,表明其在脂筏中分区。突变跨膜区的一个碱性氨基酸串(氨基酸 71-75:KKGRR)会破坏与去污剂抗性膜部分的关联,并且当在 COS-1 细胞中共转染时也会影响 ClC-6 和 ClC-7 的分离。
我们得出结论,人类 ClC-6 是一种内体糖蛋白,它在去污剂抗性脂质域中分区。内源性(晚期内体)与过表达(早期和再循环内体)ClC-6 的差异分拣类似于其他晚期内体/溶酶体膜蛋白(例如 LIMP II),并且与 ClC-6 在早期内体和晚期内体中的最终目的地之间的限速分拣步骤一致。
Zotero 插件
