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棉花籽过氧化氢酶过氧化物酶体靶向信号的鉴定

Identification of the peroxisomal targeting signal for cottonseed catalase.

作者信息

Mullen R T, Lee M S, Trelease R N

机构信息

Department of Botany, Arizona State University, Tempe 85287-1601, USA.

出版信息

Plant J. 1997 Aug;12(2):313-22. doi: 10.1046/j.1365-313x.1997.12020313.x.

DOI:10.1046/j.1365-313x.1997.12020313.x
PMID:9301084
Abstract

Catalase is a ubiquitous peroxisomal matrix enzyme, yet the molecular targeting signal(s) for sorting it in plant cells has not been defined. The most common peroxisome targeting signal (PTS) is a C-terminal tripeptide composed of a conserved SKL motif (type 1 PTS). The PTS for cottonseed catalase (Ccat) was elucidated in this study from immunofluorescence microscopic analyses of tobacco BY-2 suspension cells serving as an in vivo import system. To distinguish biolistically introduced Ccat from endogenous tobacco catalase, Ccat was hemagglutinin (HA)epitope-tagged at its N-terminus. Bombardment with HA-Ccat resulted in the import of Ccat into glyoxysomes, the specialized type of peroxisome in BY-2 cells. The C-terminal tripeptide of Ccat, PSI, is necessary for import. Evidence for this were mislocalizations to the cytosol of PSI-truncated Ccat and AGV-substituted (for PSI) Ccat. PSI-COOH, however, was not sufficient to re-route chloramphenicol acetyltransferase (CAT) from the cytosol to glyoxysomes, whereas the Ccat tetrapeptide RPSI-COOH was sufficient. Surprisingly, substitution of K (common at the fourth position in other plant catalases) for the R (CAT-KPSI) decreased import efficiency. However, substitution of K did not affect import, when additional upstream residues in Ccat were included (e.g. CAT-NVKPSI). Other evidence for the importance of upstream residues comprised abolishment of Ccat import due to substitutions with non-conserved residues (e.g. -AGVNVRPSI for -SRLNVRPSI). These data indicate that Ccat is sorted to plant peroxisomes by a degenerate type 1 PTS (PSI-COOH) whose residues are functionally dependent on a strict context of adjacent C-terminal amino acid residues.

摘要

过氧化氢酶是一种普遍存在的过氧化物酶体基质酶,但在植物细胞中对其进行分选的分子靶向信号尚未明确。最常见的过氧化物酶体靶向信号(PTS)是由保守的SKL基序组成的C端三肽(1型PTS)。本研究通过将烟草BY-2悬浮细胞作为体内导入系统进行免疫荧光显微镜分析,阐明了棉籽过氧化氢酶(Ccat)的PTS。为了将生物弹轰击导入的Ccat与内源性烟草过氧化氢酶区分开来,Ccat在其N端带有血凝素(HA)表位标签。用HA-Ccat进行轰击导致Ccat导入乙醛酸循环体,这是BY-2细胞中过氧化物酶体的特殊类型。Ccat的C端三肽PSI是导入所必需的。PSI截短的Ccat和AGV替代(替代PSI)的Ccat定位于细胞质中的错误定位证明了这一点。然而,PSI-COOH不足以将氯霉素乙酰转移酶(CAT)从细胞质重新引导至乙醛酸循环体,而Ccat四肽RPSI-COOH则足够。令人惊讶的是,将其他植物过氧化氢酶中常见的第四位的K替换为R(CAT-KPSI)会降低导入效率。然而,当包含Ccat中额外的上游残基时(例如CAT-NVKPSI),K的替换并不影响导入。上游残基重要性的其他证据包括,由于用非保守残基替代(例如-SRLNVRPSI替换为-AGVNVRPSI)导致Ccat导入被废除。这些数据表明,Ccat通过一种简并的1型PTS(PSI-COOH)被分选到植物过氧化物酶体,其残基在功能上依赖于相邻C端氨基酸残基的严格背景。

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Identification of the peroxisomal targeting signal for cottonseed catalase.棉花籽过氧化氢酶过氧化物酶体靶向信号的鉴定
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