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铰链区长度和组成对人IgA被多种细菌IgA1蛋白酶切割敏感性的影响。

The influences of hinge length and composition on the susceptibility of human IgA to cleavage by diverse bacterial IgA1 proteases.

作者信息

Senior Bernard W, Woof Jenny M

机构信息

Division of Pathology and Neuroscience, University of Dundee Medical School, Ninewells Hospital, Dundee, United Kingdom.

出版信息

J Immunol. 2005 Jun 15;174(12):7792-9. doi: 10.4049/jimmunol.174.12.7792.

DOI:10.4049/jimmunol.174.12.7792
PMID:15944283
Abstract

The influences of IgA hinge length and composition on its susceptibility to cleavage by bacterial IgA1 proteases were examined using a panel of IgA hinge mutants. The IgA1 proteases of Streptococcus pneumoniae, Streptococcus sanguis strains SK4 and SK49, Neisseria meningitidis, Neisseria gonorrhoeae, and Haemophilus influenzae cleaved IgA2-IgA1 half hinge, an Ab featuring half of the IgA1 hinge incorporated into the equivalent site in IgA1 protease-resistant IgA2, whereas those of Streptococcus mitis, Streptococcus oralis, and S. sanguis strain SK1 did not. Hinge length reduction by removal of two of the four C-terminal proline residues rendered IgA2-IgA1 half hinge resistant to all streptococcal IgA1 metalloproteinases but it remained sensitive to cleavage by the serine-type IgA1 proteases of Neisseria and Haemophilus spp. The four C-terminal proline residues could be substituted by alanine residues or transferred to the N-terminal extremity of the hinge without affect on the susceptibility of the Ab to cleavage by serine-type IgA1 proteases. However, their removal rendered the Ab resistant to cleavage by all the IgA1 proteases. We conclude that the serine-type IgA1 proteases of Neisseria and Haemophilus require the Fab and Fc regions to be separated by at least ten (or in the case of N. gonorrhoeae type I protease, nine) amino acids between Val(222) and Cys(241) (IgA1 numbering) for efficient access and cleavage. By contrast, the streptococcal IgA1 metalloproteinases require 12 or more appropriate amino acids between the Fab and Fc to maintain a minimum critical distance between the scissile bond and the start of the Fc.

摘要

利用一组IgA铰链突变体研究了IgA铰链长度和组成对其被细菌IgA1蛋白酶切割敏感性的影响。肺炎链球菌、血链球菌SK4和SK49菌株、脑膜炎奈瑟菌、淋病奈瑟菌及流感嗜血杆菌的IgA1蛋白酶可切割IgA2-IgA1半铰链,即一种将IgA1铰链的一半整合到对IgA1蛋白酶有抗性的IgA2等效位点的抗体,而缓症链球菌、口腔链球菌及血链球菌SK1菌株的IgA1蛋白酶则不能。去除四个C末端脯氨酸残基中的两个使铰链长度缩短,从而使IgA2-IgA1半铰链对所有链球菌IgA1金属蛋白酶具有抗性,但它对奈瑟菌属和嗜血杆菌属的丝氨酸型IgA1蛋白酶的切割仍敏感。四个C末端脯氨酸残基可被丙氨酸残基取代或转移至铰链的N末端,而不影响该抗体对丝氨酸型IgA1蛋白酶切割的敏感性。然而,去除这些残基使该抗体对所有IgA1蛋白酶的切割具有抗性。我们得出结论,奈瑟菌属和嗜血杆菌属的丝氨酸型IgA1蛋白酶需要Fab和Fc区域在Val(222)和Cys(241)(IgA1编号)之间至少相隔十个(对于淋病奈瑟菌I型蛋白酶则为九个)氨基酸,以便有效接近并切割。相比之下,链球菌IgA1金属蛋白酶需要Fab和Fc之间有12个或更多合适的氨基酸,以维持切割键与Fc起始部位之间的最小临界距离。

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