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斯氏按蚊中肠羧肽酶A的克隆、特性鉴定及传播阻断潜力

Cloning, characterization and transmission blocking potential of midgut carboxypeptidase A in Anopheles stephensi.

作者信息

VenkatRao V, Kumar Surendra K, Sridevi P, Muley Vijaykumar Yogesh, Chaitanya R K

机构信息

Department of Animal Biology, School of Life Sciences, University of Hyderabad, Hyderabad 500046, India.

Department of Biotechnology, Indira Gandhi National Tribal University, Amarkantak, 484224, India.

出版信息

Acta Trop. 2017 Apr;168:21-28. doi: 10.1016/j.actatropica.2016.12.035. Epub 2017 Jan 10.

DOI:10.1016/j.actatropica.2016.12.035
PMID:28087198
Abstract

Transmission-blocking vaccines (TBV) interrupt malaria parasite transmission and hence form an important component for malaria eradication. Mosquito midgut exopeptidases such as aminopeptidase N & carboxypeptidase B have demonstrated TBV potential. In the present study, we cloned and characterized carboxypeptidase A (CPA) from the midgut of an important malarial vector, Anopheles stephensi. ClustalW amino acid alignment and in silico 3-dimensional structure analysis of CPA predicted the presence of active sites involved in zinc and substrate binding that are conserved among all the known mosquito species. Real-time PCR analysis demonstrated that CPA is predominantly expressed in the midgut throughout the mosquito life cycle and that this gene is significantly elevated in P. berghei-infected mosquitoes compared to uninfected blood-fed controls. The high midgut CPA activity correlated with the prominent mRNA levels observed. Peptide-based anti-CPA antibodies were raised that cross-reacted specifically to ∼48kDa and ∼37kDa bands, which correspond to zymogen and active forms of CPA. Further, the addition of CPA-directed antibodies to P. berghei-containing blood meal significantly reduced the mosquito infection rate in the test group compared to control and blocked the parasite development in the midgut. These results support further development of A. stephensi CPA as a candidate TBV.

摘要

传播阻断疫苗(TBV)可中断疟原虫传播,因此是疟疾根除的重要组成部分。蚊中肠外肽酶如氨肽酶N和羧肽酶B已显示出具有传播阻断疫苗的潜力。在本研究中,我们从重要疟疾媒介斯氏按蚊的中肠中克隆并鉴定了羧肽酶A(CPA)。CPA的ClustalW氨基酸比对和计算机三维结构分析预测,在所有已知蚊种中都存在参与锌和底物结合的活性位点。实时PCR分析表明,CPA在蚊子整个生命周期中主要在中肠表达,并且与未感染的血饲对照相比,该基因在感染伯氏疟原虫的蚊子中显著升高。中肠中较高的CPA活性与观察到的显著mRNA水平相关。制备了基于肽的抗CPA抗体,该抗体与约48kDa和约37kDa条带发生特异性交叉反应,这两条带分别对应于CPA的酶原形式和活性形式。此外,与对照组相比,向含有伯氏疟原虫的血餐中添加CPA定向抗体显著降低了试验组蚊子的感染率,并阻断了中肠内寄生虫的发育。这些结果支持将斯氏按蚊CPA进一步开发为候选传播阻断疫苗。

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