Photoinactivation of the Staphylococcus aureus Lactose-Specific EIICB Phosphotransferase Component with p-azidophenyl-β-D-Galactoside and Phosphorylation of the Covalently Bound Substrate.

IF 1.2 Q2 Biochemistry, Genetics and Molecular Biology Journal of Molecular Microbiology and Biotechnology Pub Date : 2018-01-01 Epub Date: 2018-12-06 DOI:10.1159/000494433
Gina Sossna-Wunder, Wolfgang Hengstenberg, Pierre Briozzo, Josef Deutscher
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引用次数: 3

Abstract

Background: The phosphoenolpyruvate (PEP):lactose phosphotransferase system of Staphylococcus aureus transports and phosphorylates lactose and various phenylgalactosides. Their phosphorylation is catalyzed by the Cys476-phosphorylated EIIB domain of the lactose-specific permease enzyme IICB (EIICBLac). Phosphorylation causes the release of galactosides bound to the EIIC domain into the cytoplasm by a mechanism not yet understood.

Results: Irradiation of a reaction mixture containing the photoactivatable p-azidophenyl-β-D-galactopyranoside and EIICBLac with UV light caused a loss of EIICBLac activity. Nevertheless, photoinactivated EIICBLac could still be phosphorylated with [32P]PEP. Proteolysis of photoinactivated [32P]P-EIICBLac with subtilisin provided an 11-kDa radioactive peptide. Only the sequence of its first three amino acids (-H-G-P-, position 245-247) could be determined. They are part of the substrate binding pocket in EIICs of the lactose/cellobiose PTS family. Surprisingly, while acid treatment caused hydrolysis of the phosphoryl group in active [32P]P∼EIICBLac, photoinactivated [32P]P-EIICBLac remained strongly phosphorylated.

Conclusion: Phosphorylation of the -OH group at C6 of p-nitrenephenyl-β-D-galactopyranoside covalently bound to EIICLac by the histidyl-phosphorylated [32P]P∼EIIBLac domain is a likely explanation for the observed acid resistance. Placing p-nitrenephenyl-β-D-galactopyranoside into the active site of modelled EIICLac suggested that the nitrene binds to the -NH- group of Ser248, which would explain why no sequence data beyond Pro247could be obtained.

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对叠氮苯基-β- d -半乳糖苷对金黄色葡萄球菌乳糖特异性EIICB磷酸转移酶组分的光失活及共价结合底物的磷酸化
背景:金黄色葡萄球菌的磷酸烯醇丙酮酸(PEP):乳糖磷酸转移酶系统转运和磷酸化乳糖和各种苯半乳糖苷。它们的磷酸化是由cys476磷酸化的乳糖特异性渗透酶IICB (EIICBLac)的EIIB结构域催化的。磷酸化导致与EIIC结构域结合的半乳糖苷释放到细胞质中,其机制尚不清楚。结果:紫外光照射含有可光活化的对叠氮苯基-β- d -半乳糖苷和EIICBLac的反应混合物,导致EIICBLac活性丧失。然而,光失活的EIICBLac仍然可以被[32P]PEP磷酸化。用枯草菌素对光失活的[32P]P-EIICBLac进行蛋白水解,得到11 kda的放射性肽。仅能确定其前三个氨基酸(- h - g - p -,位置245-247)的序列。它们是乳糖/纤维素糖PTS家族EIICs中底物结合袋的一部分。令人惊讶的是,虽然酸处理导致活性[32P]P ~ EIICBLac的磷酸化基团水解,但光灭活的[32P]P-EIICBLac仍然被强烈磷酸化。结论:通过组氨酸磷酸化的[32P]P ~ EIIBLac结构域与EIICLac共价结合的对硝基苯-β- d -半乳糖苷C6的-OH基团磷酸化可能是观察到的耐酸性的一个解释。将对硝基苯-β- d -半乳糖苷置于模拟EIICLac的活性位点表明,硝基苯与Ser248的- nhh -基团结合,这可以解释为什么没有获得pro247以外的序列数据。
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来源期刊
Journal of Molecular Microbiology and Biotechnology
Journal of Molecular Microbiology and Biotechnology 生物-生物工程与应用微生物
CiteScore
3.90
自引率
0.00%
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0
审稿时长
>12 weeks
期刊介绍: We are entering a new and exciting era of microbiological study and application. Recent advances in the now established disciplines of genomics, proteomics and bioinformatics, together with extensive cooperation between academic and industrial concerns have brought about an integration of basic and applied microbiology as never before.
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