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无需重折叠或激活即可直接产生功能性基质金属蛋白酶-14及其在体外抑制试验中的应用。

Direct production of functional matrix metalloproteinase--14 without refolding or activation and its application for in vitro inhibition assays.

作者信息

Nam Dong Hyun, Ge Xin

机构信息

Department of Chemical and Environmental Engineering, University of California, 900 University Ave Riverside, Riverside, 92521, California.

出版信息

Biotechnol Bioeng. 2016 Apr;113(4):717-23. doi: 10.1002/bit.25840. Epub 2015 Oct 7.

Abstract

Human matrix metalloproteinase (MMP)-14, a membrane-bound zinc endopeptidase, is one of the most important cancer targets because it plays central roles in tumor growth and invasion. Large amounts of active MMP-14 are required for cancer research and the development of chemical or biological MMP-14 inhibitors. Current methods of MMP-14 production through refolding and activation are labor-intensive, time-consuming, and often associated with low recovery rates, lot-to-lot variation and heterogeneous products. Here, we report direct production of the catalytic domain of MMP-14 in the periplasmic space of Escherichia coli. 0.5 mg/L of functional MMP-14 was produced without tedious refolding or problematic activation process. MMP-14 prepared by simple periplasmic treatment can be readily utilized to evaluate the potencies of chemical and antibody-based inhibitors. Furthermore, co-expression of both MMP-14 and antibody Fab fragments in the periplasm facilitated inhibitory antibody screening by avoiding purification of MMP-14 or Fabs. We expect this MMP-14 expression strategy can expedite the development of therapeutic drugs targeting MMPs with biological significance.

摘要

人基质金属蛋白酶(MMP)-14是一种膜结合锌内肽酶,是最重要的癌症靶点之一,因为它在肿瘤生长和侵袭中起核心作用。癌症研究以及化学或生物MMP-14抑制剂的开发需要大量活性MMP-14。目前通过重折叠和激活来生产MMP-14的方法劳动强度大、耗时,且常常伴随着低回收率、批次间差异以及产物不均一。在此,我们报道了在大肠杆菌周质空间中直接生产MMP-14的催化结构域。无需繁琐的重折叠或有问题的激活过程,即可产生0.5mg/L的功能性MMP-14。通过简单的周质处理制备的MMP-14可很容易地用于评估基于化学和抗体的抑制剂的效力。此外,通过避免MMP-14或Fab片段的纯化,在周质中共表达MMP-14和抗体Fab片段有助于抑制性抗体的筛选。我们期望这种MMP-14表达策略能够加速具有生物学意义的靶向MMPs治疗药物的开发。

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