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非洲犀牛心肌肌钙蛋白I诊断表位的遗传特征分析

Genetic characterization of diagnostic epitopes of cardiac troponin I in African rhinoceros.

作者信息

Rautenbach Yolandi, Parsons Sven D C, Loots Angelika K, Goddard Amelia, Meyer Leith C R, Buss Peter E, Hooijberg Emma H

机构信息

Department of Companion Animal Clinical Studies, Faculty of Veterinary Science, University of Pretoria, Pretoria, Onderstepoort, South Africa.

Centre for Veterinary Wildlife Research, Faculty of Veterinary Science, University of Pretoria, Pretoria, Onderstepoort, South Africa.

出版信息

J Vet Diagn Invest. 2025 Mar;37(2):263-271. doi: 10.1177/10406387241305323. Epub 2024 Dec 26.

Abstract

African rhinoceros undergo chemical immobilization and prolonged transport during translocations for conservation purposes and, hence, experience several pathophysiologic changes, including skeletal muscle injury. Potential concurrent myocardial injury has not been investigated due to a lack of validated immunoassays. We aimed to use inferred cardiac troponin I (cTnI) amino acid sequences of southern white () and southern-central black () rhinoceros to assess the potential usefulness of several commercial cTnI immunoassays for detecting cTnI in African rhinoceros. We extracted RNA from the myocardium of deceased rhinoceros (2 white, 1 black rhinoceros) followed by primer design, cDNA synthesis via RT-PCR, and Sanger sequencing. The inferred cTnI amino acid sequences were obtained from the mRNA transcript sequences. The homology of epitope binding sites recognized by capture and detection antibodies in 6 human immunoassays was visually evaluated using aligned inferred rhinoceros cTnI amino acid sequences. Percentage identity between white and black rhinoceros cDNA nucleotide sequences was 99%; inferred amino acid sequences were identical. There were 5 amino acid differences between humans and rhinoceros in the epitope binding sites of immunoassay antibodies; 5 assays contained antibodies against epitopes that were not conserved. For one assay, the single capture antibody targeted a short heterologous epitope (residue 87-91), and cross-reactivity with rhinoceros cTnI was deemed unlikely. For the other 5 assays, complete antibody-epitope homology, or the inclusion of multiple detection or capture antibodies, or targeting of long epitopes, indicated that these assays could be suitable for further investigation of cTnI measurement in African rhinoceros.

摘要

出于保护目的,非洲犀牛在转移过程中会经历化学固定和长时间运输,因此会出现多种病理生理变化,包括骨骼肌损伤。由于缺乏经过验证的免疫测定方法,潜在的并发心肌损伤尚未得到研究。我们旨在利用南方白犀牛和中南部黑犀牛的推断心肌肌钙蛋白I(cTnI)氨基酸序列,评估几种商用cTnI免疫测定方法在检测非洲犀牛cTnI方面的潜在实用性。我们从死亡犀牛(2头白犀牛、1头黑犀牛)的心肌中提取RNA,随后进行引物设计、通过逆转录聚合酶链反应合成cDNA以及桑格测序。从mRNA转录本序列中获得推断的cTnI氨基酸序列。使用比对后的推断犀牛cTnI氨基酸序列,直观评估6种人类免疫测定方法中捕获抗体和检测抗体识别的表位结合位点的同源性。白犀牛和黑犀牛cDNA核苷酸序列之间的同一性百分比为99%;推断的氨基酸序列相同。在免疫测定抗体的表位结合位点,人类和犀牛之间有5个氨基酸差异;5种测定方法包含针对非保守表位的抗体。对于一种测定方法,单一捕获抗体靶向一个短的异源表位(第87 - 91位残基),与犀牛cTnI的交叉反应性被认为不太可能。对于其他5种测定方法,完全的抗体 - 表位同源性、包含多种检测或捕获抗体或靶向长表位,表明这些测定方法可能适合进一步研究非洲犀牛中cTnI的测量。

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