使用开发的多克隆抗体和一步式 RT-PCR 检测法优化 DAC-ELISA 和 IC-RT-PCR,以检测印度旁遮普邦金诺橙中的印度柑橘环斑病毒。

IF 2.2 4区 医学 Q3 BIOCHEMICAL RESEARCH METHODS
Aniket Angira , V.K. Baranwal , Aashish Ranjan , Nandlal Choudhary
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引用次数: 0

摘要

印度柑橘环斑病毒(ICRSV)是曼达病毒属的一种病毒,会导致柑橘环斑病,影响金诺橙的质量和产量。在植物出现明显症状之前,早期准确的检测方法至关重要。本研究从受感染的金诺组织中扩增出 507bp 的部分外壳蛋白基因(pCPG)片段,克隆到 pET28a 载体中,并转化到大肠杆菌 BL21(DE3) 细胞中。在 IPTG 诱导下,细胞过量表达了约 23kDa 的重组部分衣壳蛋白(rpCP)。经抗 His 抗体 Western 印迹验证,rpCP 被用于在兔子身上产生 ICRSV 特异性多克隆抗体(PAb)。通过 DAC-ELISA 和 IC RT-PCR 检测,以 1:1000 稀释度优化的多克隆抗体成功检测出感染金诺桔叶提取物中的 ICRSV。通过 DAC-ELISA 和 IC-RT-PCR,在稀释至 1:640 和 1:10240 (w/v,g mL-1)的样品中分别可检测到 ICRSV。此外,还对一步 RT-PCR 检测进行了优化,从金橘叶片中提取的总 RNA 中扩增出 507bp pCPG 片段,稀释度达到 1:5120(w/v,g mL-1),从而证实了 ICRSV 的存在。结果表明,IC-RT-PCR 的灵敏度分别比 DAC-ELISA 和一步 RT-PCR 方法高出 16 倍和 2 倍。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Optimization of DAC-ELISA and IC-RT-PCR using the developed polyclonal antibody and one-step RT-PCR assays for detection of Indian citrus ringspot virus in kinnow orange of Punjab, India

Indian citrus ringspot virus (ICRSV), a member of the Mandarivirus genus, causes citrus ringspot disease, impacting kinnow orange quality and yield. Early and accurate detection methods are crucial before visible symptoms manifest in plants. In this study, a 507 bp partial coat protein gene (pCPG) segment was amplified from infected kinnow leaf tissues, cloned into a pET28a vector, and transformed into E. coli BL21(DE3) cells. Induced with IPTG, the cells overexpressed a recombinant partial coat protein (rpCP) of approximately 23 kDa, purified using Ni-NTA resin via affinity chromatography. Validated in western blot with an anti-His antibody, rpCP was used to generate an ICRSV-specific polyclonal antibody (PAb) in rabbits. PAb, optimized at 1:1000 dilution, successfully detected ICRSV in infected kinnow orange leaf extracts via DAC-ELISA and IC-RT-PCR assays. ICRSV was detectable in sample dilutions up to 1:640 and 1:10240 (w/v, g mL−1) by DAC-ELISA and IC-RT-PCR, respectively. One-step RT-PCR assays were also optimized, confirming the presence of ICRSV by amplifying a 507 bp pCPG fragment from total RNA extracted from kinnow orange leaves, with dilution up to 1:5120 (w/v, g mL−1). The result demonstrated that IC-RT-PCR has a 16-fold and 2-fold higher sensitivity than DAC-ELISA and one-step RT-PCR assays.

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来源期刊
CiteScore
5.80
自引率
0.00%
发文量
209
审稿时长
41 days
期刊介绍: The Journal of Virological Methods focuses on original, high quality research papers that describe novel and comprehensively tested methods which enhance human, animal, plant, bacterial or environmental virology and prions research and discovery. The methods may include, but not limited to, the study of: Viral components and morphology- Virus isolation, propagation and development of viral vectors- Viral pathogenesis, oncogenesis, vaccines and antivirals- Virus replication, host-pathogen interactions and responses- Virus transmission, prevention, control and treatment- Viral metagenomics and virome- Virus ecology, adaption and evolution- Applied virology such as nanotechnology- Viral diagnosis with novelty and comprehensive evaluation. We seek articles, systematic reviews, meta-analyses and laboratory protocols that include comprehensive technical details with statistical confirmations that provide validations against current best practice, international standards or quality assurance programs and which advance knowledge in virology leading to improved medical, veterinary or agricultural practices and management.
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