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带有KDEL尾的半胱氨酸蛋白酶(巯基内肽酶)的C末端KDEL序列参与KDEL囊泡的形成以及巯基内肽酶的有效液泡运输。

C-terminal KDEL sequence of a KDEL-tailed cysteine proteinase (sulfhydryl-endopeptidase) is involved in formation of KDEL vesicle and in efficient vacuolar transport of sulfhydryl-endopeptidase.

作者信息

Okamoto Takashi, Shimada Tomoo, Hara-Nishimura Ikuko, Nishimura Mikio, Minamikawa Takao

机构信息

Department of Biological Sciences, Tokyo Metropolitan University, Hachioji, Tokyo, 192-0397 Japan.

出版信息

Plant Physiol. 2003 Aug;132(4):1892-900. doi: 10.1104/pp.103.021147.

Abstract

Sulfhydryl-endopeptidase (SH-EP) is a papain-type vacuolar proteinase expressed in cotyledons of germinated Vigna mungo seeds, and the enzyme possesses a C-terminal propeptide containing KDEL tail, an endoplasmic reticulum retention signal for soluble proteins. SH-EP is transported to vacuoles via a KDEL vesicle (KV) through a Golgi complex-independent route. To see the function of the KDEL sequence of SH-EP, wild-type SH-EP and its KDEL deletion mutant (SH-EPDeltaKDEL) were heterologously expressed in Arabidopsis and in cultured tobacco Bright Yellow 2 cells, and their intracellular transport pathways and localizations were analyzed. A combination of the results from analyses for transformed Arabidopsis and tobacco (Nicotiana tabacum) cells indicated that wild-type SH-EP is packed into KV-like vesicles through the KDEL sequence and is transported to vacuoles in the cells of transformants. In contrast, KV was not formed/induced in the cells expressing SH-EPDeltaKDEL, and the mutant protein was mainly secreted. Therefore, the C-terminal KDEL sequence of the KDEL-tailed cysteine proteinase is thought to be involved in the formation of KV, and in the efficient vacuolar transport of the proteins through KV.

摘要

巯基内肽酶(SH-EP)是一种在发芽的绿豆种子子叶中表达的木瓜蛋白酶型液泡蛋白酶,该酶具有一个包含KDEL尾的C末端前肽,这是一种可溶性蛋白质的内质网保留信号。SH-EP通过独立于高尔基体复合体的途径经由KDEL囊泡(KV)转运至液泡。为了探究SH-EP的KDEL序列的功能,野生型SH-EP及其KDEL缺失突变体(SH-EPΔKDEL)在拟南芥和培养的烟草Bright Yellow 2细胞中进行了异源表达,并分析了它们的细胞内转运途径和定位。对转化的拟南芥和烟草(烟草)细胞的分析结果表明,野生型SH-EP通过KDEL序列被包装到类似KV的囊泡中,并在转化体的细胞中转运至液泡。相反,在表达SH-EPΔKDEL的细胞中未形成/诱导KV,且突变蛋白主要被分泌。因此,KDEL尾半胱氨酸蛋白酶的C末端KDEL序列被认为参与了KV的形成,以及蛋白质通过KV向液泡的高效转运。

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