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Pokeweed antiviral protein (PAP) mutations which permit E.coli growth do not eliminate catalytic activity towards prokaryotic ribosomes.

机译:允许大肠杆菌生长的商陆抗病毒蛋白(PAP)突变不会消除对原核生物核糖体的催化活性。

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摘要

Pokeweed antiviral protein (PAP) has N-glycosidase activity towards both eukaryotic and prokaryotic ribosomes. This is in marked contrast with the A chains of type 2 ribosome inactivating proteins (RIPs) such as ricin and abrin, which inactivate only eukaryotic ribosomes. A recent report described spontaneous mutations in PAP that implicated specific amino acids to be involved in determining the activity of PAP towards prokaryotic ribosomes. As part of an ongoing study into RIP--ribosome interactions these mutations were specifically recreated in a PAP clone encoding the mature 262 amino acid PAP sequence. Mutants were tested for their N-glycosidase activity by analysing the integrity of eukaryotic and prokaryotic ribosomes after mutant protein expression. Mutations of F196Y and K211R, either individually or within the same clone, were active toward both classes of ribosome, indicating that these amino acid positions are not involved in differentiating ribosomal substrates. Mutation R68G led to a protein that appeared to be inactive towards prokaryotic ribosomes, but also very poorly active towards eukaryotic ribosomes. This mutation is currently under further investigation.
机译:商陆抗病毒蛋白(PAP)对真核和原核核糖体均具有N-糖苷酶活性。这与2型核糖体失活蛋白(RIP)的A链(如蓖麻蛋白和阿布林)形成鲜明对比,后者仅使真核生物核糖体失活。最近的一份报告描述了PAP中的自发突变,涉及特定氨基酸参与确定PAP对原核生物的活性。作为正在进行的RIP-核糖体相互作用研究的一部分,这些突变是在编码成熟的262个氨基酸的PAP序列的PAP克隆中特异重建的。通过分析突变蛋白表达后真核和原核核糖体的完整性,测试突变体的N-糖苷酶活性。 F196Y和K211R的突变,无论是单独还是在同一克隆中,都对两类核糖体均具有活性,表明这些氨基酸位置不参与区分核糖体底物。突变R68G产生了一种蛋白质,该蛋白质似乎对原核生物没有活性,但对真核生物却缺乏活性。该突变目前正在进一步研究中。

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