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大肠杆菌磷酸转移酶系统中的可溶性糖通透酶:体内存在两种物理性质不同的蛋白质形式的证据。

Soluble sugar permeases of the phosphotransferase system in Escherichia coli: evidence for two physically distinct forms of the proteins in vivo.

作者信息

Aboulwafa Mohammad, Saier Milton H

机构信息

Division of Biological Sciences, University of California at San Diego, La Jolla, CA 92093-0116, USA.

出版信息

Mol Microbiol. 2003 Apr;48(1):131-41. doi: 10.1046/j.1365-2958.2003.03394.x.

Abstract

The bacterial phosphoenolpyruvate-dependent phosphotransferase system (PTS) consists of a set of cytoplasmic energy-coupling proteins and various integral membrane permeases/sugar phosphotransferases, each specific for a different sugar. We have conducted biochemical analyses of three PTS permeases (enzymes II), the glucose permease (IIGlc), the mannitol permease (IIMtl) and the mannose permease (IIMan). These enzymes each catalyse two vectorial/chemical reactions, sugar phosphorylation using phosphoenolpyruvate (PEP) as the phosphoryl donor, dependent on enzyme I, HPr and IIA as well as IIBC (the PEP reaction), and transphosphorylation using a sugar phosphate (glucose-6-P for IIGlc and IIMan; mannitol-1-P for IIMtl) as the phosphoryl donor, dependent only on IIBC (the TP reaction). When crude extracts of French-pressed or osmotically shocked Escherichia coli cells are centrifuged in an ultracentrifuge at high speed, 5-20% of the enzyme II activity remains in the high-speed supernatant, and passage through a gel filtration column gives two activity peaks, one in the void volume exhibiting high PEP-dependent and TP activities, and a second included peak with high PEP-dependent activity and high (IIMan), moderate (IIGlc) or negligible (IIMtl) TP activities. Both log and stationary phase cells exhibit comparable relative amounts of pelletable and soluble enzyme II activities, but long-term exposure of cells to chloramphenicol results in selective loss of the soluble fraction with retention of much of the pelleted activity concomitant with extensive protein degradation. Short-term exposure of cells to chloramphenicol results in increased activities in both fractions, possibly because of increased lipid association, with more activation in the soluble fraction than in the pelleted fraction. Western blot analyses show that the soluble IIGlc exhibits a subunit size of about 45 kDa, and all three soluble enzymes II elute from the gel filtration column with apparent molecular weights of 40-50 kDa. We propose that enzymes II of the PTS exist in two physically distinct forms in the E. coli cell, one tightly integrated into the membrane and one either soluble or loosely associated with the membrane. We also propose that the membrane-integrated enzymes II are largely dimeric, whereas the soluble enzymes II, retarded during passage through a gel filtration column, are largely monomeric.

摘要

细菌磷酸烯醇丙酮酸依赖性磷酸转移酶系统(PTS)由一组细胞质能量偶联蛋白和各种整合膜通透酶/糖磷酸转移酶组成,每种酶对不同的糖具有特异性。我们对三种PTS通透酶(酶II)进行了生化分析,即葡萄糖通透酶(IIGlc)、甘露醇通透酶(IIMtl)和甘露糖通透酶(IIMan)。这些酶各自催化两个向量/化学反应,以磷酸烯醇丙酮酸(PEP)作为磷酰基供体进行糖磷酸化,这依赖于酶I、HPr和IIA以及IIBC(PEP反应),以及以糖磷酸(IIGlc和IIMan为葡萄糖-6-磷酸;IIMtl为甘露醇-1-磷酸)作为磷酰基供体进行转磷酸化,仅依赖于IIBC(TP反应)。当对经法国压榨或渗透压休克处理的大肠杆菌细胞的粗提物进行超速离心时,5% - 20%的酶II活性保留在高速上清液中,并且通过凝胶过滤柱会出现两个活性峰,一个在空体积中,表现出高的PEP依赖性和TP活性,另一个包含峰具有高的PEP依赖性活性和高(IIMan)、中等(IIGlc)或可忽略不计(IIMtl)的TP活性。对数期和稳定期细胞的可沉淀和可溶性酶II活性的相对量相当,但细胞长期暴露于氯霉素会导致可溶性部分选择性丧失,同时保留大部分沉淀活性,并伴有大量蛋白质降解。细胞短期暴露于氯霉素会导致两个部分的活性增加。这可能是由于脂质结合增加,可溶性部分的激活比沉淀部分更多。蛋白质印迹分析表明,可溶性IIGlc的亚基大小约为45 kDa,并且所有三种可溶性酶II从凝胶过滤柱洗脱时的表观分子量为40 - 50 kDa。我们提出,PTS的酶II在大肠杆菌细胞中以两种物理上不同的形式存在,一种紧密整合到膜中,另一种是可溶性的或与膜松散结合。我们还提出,膜整合的酶II主要是二聚体,而在通过凝胶过滤柱时受阻的可溶性酶II主要是单体。

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