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Four monoclonal antibodies inhibit the recognition of arylsulphatase A by the lysosomal enzyme phosphotransferase.

机译:四种单克隆抗体可抑制溶酶体酶磷酸转移酶对芳基硫酸酯酶A的识别。

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摘要

The critical step in the sorting of lysosomal enzymes is their recognition by a phosphotransferase in the Golgi apparatus. The topogenic sequences responsible for the recognition by this enzyme have so far only been defined for the lysosomal protease cathepsin D. We have generated four monoclonal antibodies directed against lysosomal arylsulphatase A (ASA). These antibodies inhibit the recognition of ASA by the phosphotransferase in vitro and thus define a region of topogenic sequences in the ASA polypeptide. The antibodies do not interfere with the enzymic activity nor with pH-dependent dimerization of ASA. The epitopes recognized by the antibodies have been located in the second quarter of the ASA polypeptide using chimeric mouse-human ASA molecules. Three of the monoclonal antibodies bind to identical or closely adjacent epitopes, which are formed by the interaction of amino acid residues 165-184 and 202-240. The fourth antibody recognizes a different epitope within amino acids 256-265.
机译:溶酶体酶分类中的关键步骤是它们在高尔基体中被磷酸转移酶识别。迄今为止,仅由溶酶体蛋白酶组织蛋白酶D定义了负责由该酶识别的拓扑序列。我们已经产生了四种针对溶酶体芳基硫酸酯酶A(ASA)的单克隆抗体。这些抗体在体外抑制磷酸转移酶对ASA的识别,因此在ASA多肽中定义了拓扑序列的区域。抗体既不干扰酶的活性,也不干扰ASA的pH依赖性二聚。使用嵌合的小鼠-人ASA分子,抗体识别的表位位于ASA多肽的第二个四分之一处。三种单克隆抗体结合相同或紧密相邻的表位,这些表位是由氨基酸残基165-184和202-240的相互作用形成的。第四抗体识别氨基酸256-265内的不同表位。

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