结核分枝杆菌Rv2647蛋白对肺组织损伤效应的初步研究

doi:10.7655/NYDXBNSN240642

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结核分枝杆菌Rv2647蛋白对肺组织损伤效应的初步研究
DOI:
                        10.7655/NYDXBNSN240642
                    
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作者单位:1.南京医科大学第二附属医院呼吸与危重症医学科，江苏 南京 210011 ; 2.南京医科大学附属逸夫医院呼吸与危重症医学科，江苏 南京 211166 ; 3.南京医科大学附属江宁医院呼吸与危重症医学科，江苏 南京 211100 ; 4.江苏省疾病预防与控制中心慢性传染病防治所，江苏 南京 210009
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中图分类号:R521
基金项目:国家自然科学基金（82070017）

Preliminary study on the effect of Mycobacterium tuberculosis Rv2647 protein on lung injury

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1.Department of Pulmonary and Critical Care Medicine,the Second Affiliated Hospital of Nanjing Medical University,Nanjing 210011 ; 2.Department of Pulmonary and Critical Care Medicine,the Affiliated Sir Run Run Hospital ofNanjing Medical University,Nanjing 211166 ; 3.Department of Pulmonary and Critical Care Medicine,the AffiliatedJiangning Hospital of Nanjing Medical University,Nanjing 211100 ; 4.Institute of Chronic Infectious DiseasesPrevention and Control,Jiangsu Province Center for Disease Control and Prevention,Nanjing 210009 ,China

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目的：通过噬菌体重组技术分别构建结核分枝杆菌Rv2647基因的敲除株和回补株以及过表达Rv2647的耻垢分枝杆菌（Mycobacterium smegmatis，Ms），评估结核分枝杆菌Rv2647蛋白对模型鼠肺组织的损伤效应。方法：构建同源交换位点并整合到结核分枝杆菌噬菌体基因组，获取噬菌粒并将其导入Ms，构建具有同源交换位点的重组噬菌体。体外扩增获得高滴度重组噬菌体并转染结核分枝杆菌（H37Rv），37 ℃静置培养 28 d，挑取单克隆进行 PCR 验证，获得 Rv2647 基因敲除株（H37RvΔRv2647）。PCR 扩增Rv2647基因并通过无缝克隆分别将其整合到载体pMV361和pMV261多克隆位点处，获得阳性质粒后分别电转化H37RvΔRv2647和Ms，获得结核分枝杆菌回补株（H37RvΔRv2647：：Rv2647）及过表达Rv2647的耻垢分枝杆菌（Ms：：Rv2647）。分别以H37Rv、H37RvΔRv2647、H37RvΔRv2647：：Rv2647、Ms及Ms：：Rv2647的菌液经气管攻击C57BL/6小鼠，分别比较 H37Rv（30 d）与 Ms（7 d）模型鼠的存活率、肺组织细菌负荷及肺组织病理损伤程度。结果：PCR 结果显示， H37RvΔRv2647 中 Rv2647 基因缺失，而 H37RvΔRv2647：：Rv2647 及 Ms：：Rv2647 中 Rv2647 基因皆存在。H37RvΔRv2647、 H37Rv及H37RvΔRv2647：：Rv2647组模型鼠30 d存活率分别为100.00%、83.33%及83.33%；Ms和Ms：：Rv2647组模型鼠的7 d 存活率分别为100.00%和83.33%；H37RvΔRv2647组模型鼠肺组织细菌负荷（lgCFU）为（3.40±0.18），显著低于H37Rv组（3.86± 0.15，P ＜ 0.001）和H37RvΔRv2647：：Rv2647组（3.80±0.16，P ＜ 0.01）；H37RvΔRv2647组模型鼠肺组织炎症面积（%）为（4.37± 3.06），显著低于H37Rv组（62.76±14.24，P ＜ 0.001）和H37RvΔRv2647：：Rv2647组（67.37±0.45，P ＜ 0.001）；Ms组模型鼠肺组织 lgCFU为（2.53±0.16），显著低于Ms：：Rv2647组（2.81±0.13，P ＜ 0.01）；Ms组模型鼠肺组织炎症面积（%）为（5.71±1.29），显著低于 Ms：：Rv2647 组（33.13±13.84，P ＜ 0.05）。结论：成功构建了结核分枝杆菌 Rv2647 基因敲除株（H37RvΔRv2647）及回补株（H37RvΔRv2647：：Rv2647）以及过表达Rv2647的耻垢分枝杆菌（Ms：：Rv2647）。Rv2647蛋白可能通过抑制宿主对结核分枝杆菌的清除，加重了模型鼠肺组织病理损伤。

Abstract:

Objective：To constract the Rv2647-deleted strain and Rv2647-complemented strain of Mycobacterium tuberculosis（M. tb） and Rv2647-overexpressing Mycobacterium smegmatis（Ms：：Rv2647）by phage recombination technique，and to evaluate the effect of M. tb Rv2647 protein on lung injury in model mice. Methods：A homologous exchange site was constructed and integrated into the phage genomes of M. tb，producing phagemids that were introduced into Mycobacterium smegmatis（Ms）to create a recombinant phage with a homologous exchange site. High-titer recombinant phages were amplified in vitro and transfected into M. tb（H37Rv），followed by static culture at 37 ℃ for 28 d. The single clone was selected and verified by PCR，yeilding the Rv2647 - deleted strain （H37RvΔRv2647）. The Rv2647 gene was amplified by PCR and was integrated into the multiple clone sites of vector pMV361 and pMV261 through seamless cloning to obtain the positive plasmids，which were transfected into H37RvΔRv2647 and Ms to obtain the Rv2647 - complemented strain（H37RvΔRv2647：：Rv2647）and Rv2647 - overexpressing Ms（Ms：：Rv2647），respectively. The suspension of H37Rv，H37RvΔRv2647，H37RvΔRv2647：：Rv2647，Ms，and Ms：：Rv2647 were used to infect C57BL/6 mice via tracheal injection. The survival rates，lung tissue bacterial load，and pathological damage of lung tissue in model mice were compared at 7 d and 30 d，respectively. Results：The PCR showed that Rv2647 gene was missing in the H37RvΔRv2647，while it was present in the H37RvΔRv2647：：Rv2647 and Ms：：Rv2647. The 30-day survival rates of model mice infected with H37RvΔRv2647，H37Rv，and H37RvΔRv2647：：Rv2647 were 100.00%，83.33%，and 83.33%，respectively；The 7-day survival rates of model mice infected with Ms and Ms：：Rv2647 were 100.00% and 83.33%，respectively. The lung bacterial load（lgCFU）of model mice in the H37RvΔRv2647 group（3.40±0.18）was significantly lower than that of the H37Rv group（3.86±0.15），P ＜ 0.001）and the H37RvΔRv2647：：Rv2647 group（3.80±0.16），P ＜ 0.01）；The inflammation area（%）in lung tissues of the H37RvΔRv2647 group（4.37±3.06）was significantly lower than that of the H37Rv group（62.76±14.24），P ＜ 0.001）and the H37RvΔRv2647：：Rv2647 group（67.37±0.45），P ＜ 0.001）. The lung bacterial load（lgCFU）of the Ms group（2.53±0.16）was significantly lower than that of the Ms：：Rv2647 group（2.81±0.13）， P ＜ 0.01）；The inflammation area（%）in lung tissue of the Ms group（5.71±1.29）was significantly lower than that of the Ms：：Rv2647 group（33.13 ± 13.84），P ＜ 0.05）. Conclusion：The Rv2647 - deleted strain（H37RvΔRv2647）and Rv2647 - complementary strain （H37RvΔRv2647：：Rv2647）of M. tb and Rv2647-overexpressing Ms（Ms：：Rv2647）were successfully constructed. Rv2647 protein may aggravate lung injury via inhibiting host clearance of M. tb.

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金霄,陈晓林,姚静,杜兴冉,颜海豪,李国莉,冯旰珠.结核分枝杆菌Rv2647蛋白对肺组织损伤效应的初步研究[J].南京医科大学学报（自然科学版）,2024,(11):1517-1524

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收稿日期:2024-06-25
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