Journal of proteolysis最新文献

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Peptide Sequence Region That is Essential for the Interactions of the Enterotoxigenic Bacteroides fragilis Metalloproteinase II with E-cadherin. 产肠毒素的脆弱拟杆菌金属蛋白酶II与e -钙粘蛋白相互作用的肽序列区域。

Journal of proteolysis

Pub Date : 2014-12-22

Sergey A Shiryaev, Albert G Remacle, Piotr Cieplak, Alex Y Strongin

Bacteroides fragilis is a valuable anaerobic commensal and an essential component of the gut microbiome in humans. The presence of a short pathogenicity island in the genome is predominantly associated with the enterotoxigenic strains of B. fragilis. Metallopro-teinase II (MPII) and fragilysin (FRA) are the structurally related enzymes encoded by the pathogenicity island in the enterotoxigenic strains. Accordingly, there is a significant overlap between the cleavage preferences of MPII and FRA. These proteinases, however, are counter-transcribed in the bacterial genome suggesting their distinct and specialized functions in the course of infection. It is well established that FRA directly cleaves E-cadherin, a key protein of the cell-to-cell adhesion junctions in the intestinal epithelium. Counterintuitively, MPII directly binds to, rather than cleaves, E-cadherin. Structural modeling suggested that a potential E-cadherin binding site involves the C-terminal -helical region of the MPII catalytic domain. The sequence of this region is different in MPII and FRA. Here, we employed substitution mutagenesis of this C-terminal -helical region to isolate the MPII mutants with the potentially inactivated E-cadherin binding site. Overall, as a result of our modeling, mutagenesis and binding studies, we determined that the C-terminal ten residue segment is essential for the binding of MPII, but not of FRA3, to E-cadherin, and that the resulting MPII•E-cadherin complex does not impair E-cadherin-dependent cell-to-cell contacts. It is possible to envision that the putative cleavage targets of MPII should be explored not only on the host cell surface but also in B. fragilis.

脆弱拟杆菌是一种有价值的厌氧共生菌，是人类肠道微生物群的重要组成部分。基因组中短致病性岛的存在主要与产肠毒素的易碎芽孢杆菌菌株有关。金属蛋白酶II (MPII)和脆性溶素(FRA)是肠道产毒菌株致病性岛编码的结构相关酶。因此，在MPII和FRA的切割偏好之间存在显著的重叠。然而，这些蛋白酶在细菌基因组中是反转录的，这表明它们在感染过程中具有独特的特殊功能。已经证实，FRA直接切割肠上皮细胞间黏附连接的关键蛋白E-cadherin。与直觉相反，MPII直接与e -钙粘蛋白结合，而不是切割。结构建模表明，潜在的e -钙粘蛋白结合位点涉及MPII催化结构域的c端-螺旋区域。该区域在MPII和FRA中的序列不同。在这里，我们采用c端螺旋区域的替代诱变方法分离出具有潜在失活e -钙粘蛋白结合位点的MPII突变体。总的来说，通过建模、诱变和结合研究，我们确定了c端10残基片段对于MPII与E-cadherin的结合至关重要，而不是FRA3与E-cadherin的结合，并且由此产生的MPII•E-cadherin复合物不会损害E-cadherin依赖的细胞间接触。可以设想，MPII的切割靶点不仅应该在宿主细胞表面上进行探索，而且应该在脆弱芽孢杆菌中进行探索。

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