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不同形式的A型肉毒杆菌神经毒素的差异内肽酶活性:底物大小与酶活性之间的独特关系。

Differential endopeptidase activity of different forms of type A botulinum neurotoxin: A unique relationship between the size of the substrate and activity of the enzyme.

作者信息

Ambrin Ghuncha, Kumar Raj, Singh Bal Ram

机构信息

Department of Chemistry and Biochemistry, University of Massachusetts, North Dartmouth, MA, 02747, USA.

Botulinum Research Center, Institute of Advanced Sciences, Dartmouth, MA 02747, USA.

出版信息

Toxicon. 2018 Mar 15;144:34-41. doi: 10.1016/j.toxicon.2017.12.055. Epub 2018 Jan 5.

DOI:10.1016/j.toxicon.2017.12.055
PMID:29309744
Abstract

Botulinum neurotoxins (BoNTs; serotypes A-G) are metalloproteases, which cleave and inactivate cellular proteins essential for neurotransmitter release. In bacterial cultures, BoNTs are secreted as a complex of the neurotoxin and a group of neurotoxin associated proteins (NAPs). Under physiological condition (pH 7.4), this complex is believed to be dissociated to separate the neurotoxin from NAPs. BoNT consists of a 50 kDa light (L) chain (LC or catalytic domain) and a 100 kDa heavy (H) chain (or HC) linked through a disulfide bond and other non-covalent interactions. The cell intoxication involves three major steps; binding, membrane translocation and inhibition of neurotransmitter release. The last step of intoxication, endopeptidase activity, is very unique and specific that can be used for detection of the complex and isolated forms of the toxin. A fluorescent tag-labeled synthetic peptide (SNAPtide) derived from a segment of SNAP-25, an intracellular substrate of BoNT/A, is used to detect and assay the endopeptidase activity of BoNT/A. The detection of the signal is based on the change in the fluorescence energy transfer after selective cleavage of the peptide by the BoNT/A. In this report, we demonstrate that SNAPtide as a commonly used substrate widely differ in reaction with BoNT/A complex, BoNT/A, and BoNT/A light chain. These findings have implications for assays used in detection, and in screening potential inhibitors.

摘要

肉毒杆菌神经毒素(BoNTs;血清型A - G)是金属蛋白酶,可切割并使神经递质释放所必需的细胞蛋白失活。在细菌培养物中,BoNTs以神经毒素与一组神经毒素相关蛋白(NAPs)的复合物形式分泌。在生理条件(pH 7.4)下,这种复合物被认为会解离,从而将神经毒素与NAPs分开。BoNT由一条50 kDa的轻(L)链(LC或催化结构域)和一条100 kDa的重(H)链(或HC)组成,二者通过二硫键及其他非共价相互作用相连。细胞中毒涉及三个主要步骤:结合、膜转位和神经递质释放抑制。中毒的最后一步,即内肽酶活性,非常独特且具有特异性,可用于检测毒素的复合物形式和分离形式。一种源自BoNT/A细胞内底物SNAP - 25片段的荧光标签标记合成肽(SNAPtide),用于检测和测定BoNT/A的内肽酶活性。信号检测基于BoNT/A对肽进行选择性切割后荧光能量转移的变化。在本报告中,我们证明,作为常用底物的SNAPtide与BoNT/A复合物、BoNT/A和BoNT/A轻链的反应存在广泛差异。这些发现对检测及筛选潜在抑制剂的测定方法具有重要意义。

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