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alpha5 subunit in Trypanosoma brucei proteasome can self-assemble to form a cylinder of four stacked heptamer rings.

机译:布氏锥虫蛋白酶体中的alpha5亚基可以自组装形成四个堆叠的七聚体环的圆柱体。

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摘要

The proteasomes have a central role in catalysing protein degradation among both prokaryotes and eukaryotes. The 20 S proteasome constitutes their catalytic core. In studying the structure of Trypanosoma brucei 20 S proteasomes, we isolated by two-dimensional (2D) gel electrophoresis a 27 kDa subunit protein with an estimated pI of 4.7 and subjected it to mass spectrometric analysis. A tryptic peptide sequence from the protein was found identical with that of the rat alpha5 subunit. With the use of antiserum against T. brucei 20 S proteasomes to screen a T. b. rhodesiense lambda expression cDNA library, we obtained a cDNA clone encoding a full-length protein of 246 amino acid residues with a calculated molecular mass of 27174 Da and a pI of 4.71. It bears 50. 0% and 46.3% sequence identity with rat and yeast proteasome subunit alpha5 respectively, and matches all the peptide sequences derived from MS of the 2D gel-purified protein. The protein is thus designated the alpha5 subunit of T. brucei 20 S proteasome (TbPSA5). The recombinant protein, expressed in plasmid-transformed Escherichia coli, was found in a 27 kDa monomer form as well as polymerized forms with estimated molecular masses ranging from 190 to 800 kDa. Under the electron microscope, the most highly polymerized forms bear the appearance of cylinders of four-stacked heptamer rings with an estimated outer diameter of 14.5 nm and a length of 18 nm, which were immunoprecipitable by anti-(T. brucei 20 S proteasome) antiserum. In view of the documented self-assembly of the archaeon proteasome alpha subunit into double heptamer rings and the spontaneous assembly of the two alpha subunits from the 20 S proteasome of Rhodococcus erythropolis, the self-assembly of the T. brucei alpha subunit might reflect a common feature of proteasome biogenesis shared by prokaryotes and primitive eukaryotes such as the trypanosomes but apparently lost among the higher forms of eukaryote such as the yeast and the mammals.
机译:蛋白酶体在催化原核生物和真核生物中的蛋白质降解中具有重要作用。 20 S蛋白酶体构成其催化核心。在研究布鲁氏锥虫20 S蛋白酶体的结构时,我们通过二维(2D)凝胶电泳分离了一个27 kDa的亚基蛋白,其pI估计为4.7,并对其进行了质谱分析。发现该蛋白质的胰蛋白酶肽序列与大鼠alpha5亚基的相同。使用针对布鲁氏菌20 S蛋白酶体的抗血清筛选T. b。 Rhodesiense lambda表达cDNA文库,我们获得了cDNA克隆,该克隆编码246个氨基酸残基的全长蛋白,计算分子量为27174 Da,pI为4.71。它分别与大鼠和酵母蛋白酶体亚基alpha5具有50. 0%和46.3%的序列同一性,并匹配所有源自2D凝胶纯化蛋白MS的肽序列。因此,该蛋白质被称为布鲁氏菌20 S蛋白酶体(TbPSA5)的alpha5亚基。发现在质粒转化的大肠杆菌中表达的重组蛋白呈27 kDa单体形式以及聚合形式,其估计分子量为190至800 kDa。在电子显微镜下,聚合度最高的形式带有四叠七聚体环的圆柱体,其估计的外径为14.5 nm,长度为18 nm,可被抗T. brucei 20 S蛋白酶体免疫沉淀。抗血清。鉴于古细菌蛋白酶体α亚基自组装成双七聚体环以及红球红球菌20 S蛋白酶体中两个α亚基的自发组装,布鲁氏球菌α亚基的自组装可能反映了原核生物和原始的真核生物(如锥虫)共有蛋白酶体生物发生的共同特征,但显然在高级形式的真核生物(如酵母和哺乳动物)中消失了。

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