高等植物蛋白质的特异性降解系统

在细胞内功能蛋白质处于不断的合成与降解中,其中蛋白质的特异性降解是蛋白功能调节的重要机制。蛋白质的特异性降解分为泛素依赖的途径和非泛素依赖途径。在泛素依赖的降解途径中,蛋白质在泛素激活酶、泛素结合酶、泛素连接酶的作用下泛素化,然后在26S蛋白酶体中进行降解。蛋白质也可不依赖泛素被26S蛋白酶体降解,或被游离的20S蛋白酶体降解。本文主要介绍高等植物中的蛋白质特异性降解途径及特异性机制的研究进展。

New Role for an Old Rule: N-end Rule-Mediated Degradation of Ethylene Responsive Factor Proteins Governs Low Oxygen Response in Plants

The N-end rule pathway regulates protein degradation, which depends on exposed N-terminal sequences in prokaryotes and eukaryotes. In plants, conserved and specific enzymes stimulate selective proteolysis. Although a number of developmental and growth phenotypes have been reported for mutants in the N-end rule, its function has remained unrelated to specific physiological pathways. The first report of the direct involvement of the N-end rule in stress responses focused on hypoxic signaling and how the oxygen-dependent oxidation of cystein promotes the N-end rule-mediated degradation of ethylene responsive factor （ERF）-VII proteins, the master regulators of anaerobic responses. It has been suggested that plants have evolved specific mechanisms to tune ERF-VII availability in the nucleus. In this review, we speculate that ERF-VII proteins are reversibly protected from degradation via membrane sequestration. The oxidative response in plants subjected to anoxic conditions suggests that reactive oxygen and nitrogen species （reactive oxygen species and reactive nitrogen species） may interact or interfere with the N-end rule pathway-mediated response to hypoxia.

N端规则泛素E3连接酶UBR2真核表达载体的构建及验证

目的 构建N-端规则泛素E3连接酶UBR2过表达载体,并检测它在HepG2细胞中的过表达效率.方法 通过提取HepG2细胞总RNA, RT-PCR扩增UBR2基因片段,插入到pEGFP-N2载体中,构建真核表达载体pEGFP-N2-UBR2,并转染HepG2细胞,转染后利用荧光显微镜,Western印迹检测UBR2的表达情况.结果 经双酶切和测序鉴定真核表达质粒pEGFP-N2-UBR2构建正确;转染后24 h,利用荧光显微镜观察,在转染pEGFP-N2-UBR2的HepG2细胞中观察到绿色荧光蛋白,在蛋白水平可以检测到UBR2蛋白过表达.结论 成功构建pEGFP-N2-UBR2过表达载体,并在HepG2细胞中验证其过表达效率.为今后研究其在细胞生长和增殖过程中的作用奠定基础.