组氨酸激酶<bold>EnvZ</bold>调节副溶血弧菌群集性爬动和生物被膜形成的作用机制

doi:10.13343/j.cnki.wsxb.20240695

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组氨酸激酶EnvZ调节副溶血弧菌群集性爬动和生物被膜形成的作用机制
DOI:
                        10.13343/j.cnki.wsxb.20240695
                    
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作者:
                        袁艺萱袁艺萱
浙江农林大学 动物科技学院·动物医学院，浙江省畜禽绿色生态健康养殖应用技术研究重点实验室，动物健康互联网检测技术浙江省工程实验室，浙江 杭州
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吴文婷吴文婷
浙江农林大学 动物科技学院·动物医学院，浙江省畜禽绿色生态健康养殖应用技术研究重点实验室，动物健康互联网检测技术浙江省工程实验室，浙江 杭州
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陆倩陆倩
浙江农林大学 动物科技学院·动物医学院，浙江省畜禽绿色生态健康养殖应用技术研究重点实验室，动物健康互联网检测技术浙江省工程实验室，浙江 杭州
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姚宁姚宁
浙江农林大学 动物科技学院·动物医学院，浙江省畜禽绿色生态健康养殖应用技术研究重点实验室，动物健康互联网检测技术浙江省工程实验室，浙江 杭州
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周秀娟周秀娟
浙江农林大学 动物科技学院·动物医学院，浙江省畜禽绿色生态健康养殖应用技术研究重点实验室，动物健康互联网检测技术浙江省工程实验室，浙江 杭州
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钟孝俊钟孝俊
浙江农林大学 动物科技学院·动物医学院，浙江省畜禽绿色生态健康养殖应用技术研究重点实验室，动物健康互联网检测技术浙江省工程实验室，浙江 杭州
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杨梦华杨梦华
浙江农林大学 动物科技学院·动物医学院，浙江省畜禽绿色生态健康养殖应用技术研究重点实验室，动物健康互联网检测技术浙江省工程实验室，浙江 杭州
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作者单位:浙江农林大学 动物科技学院·动物医学院，浙江省畜禽绿色生态健康养殖应用技术研究重点实验室，动物健康互联网检测技术浙江省工程实验室，浙江 杭州
作者简介:袁艺萱：实验操作、数据收集和处理；吴文婷：协助实验操作、数据收集；陆倩：协助实验操作、数据处理；姚宁：协助实验操作；周秀娟：论文讨论；钟孝俊：数据处理、论文撰写和修改；杨梦华：实验设计、论文讨论和修改。
通讯作者:
中图分类号:
基金项目:国家自然科学基金(32170174, 32202804)；浙江省自然科学基金(LQ22C180002)；浙江农林大学科研发展启动基金(2013FR012, 2020FR042)

The histidine kinase EnvZ regulates the swarming motility and biofilm formation of Vibrio parahaemolyticus

Author:

YUAN Yixuan
YUAN Yixuan
Key Laboratory of Applied Technology on Green-Eco-Healthy Animal Husbandry of Zhejiang Province, Zhejiang Provincial Engineering Laboratory for Animal Health Inspection & Internet Technology, College of Animal Science and Technology & College of Veterinary Medicine, Zhejiang A&F University, Hangzhou, Zhejiang, China
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WU Wenting
WU Wenting
Key Laboratory of Applied Technology on Green-Eco-Healthy Animal Husbandry of Zhejiang Province, Zhejiang Provincial Engineering Laboratory for Animal Health Inspection & Internet Technology, College of Animal Science and Technology & College of Veterinary Medicine, Zhejiang A&F University, Hangzhou, Zhejiang, China
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LU Qian
LU Qian
Key Laboratory of Applied Technology on Green-Eco-Healthy Animal Husbandry of Zhejiang Province, Zhejiang Provincial Engineering Laboratory for Animal Health Inspection & Internet Technology, College of Animal Science and Technology & College of Veterinary Medicine, Zhejiang A&F University, Hangzhou, Zhejiang, China
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YAO Ning
YAO Ning
Key Laboratory of Applied Technology on Green-Eco-Healthy Animal Husbandry of Zhejiang Province, Zhejiang Provincial Engineering Laboratory for Animal Health Inspection & Internet Technology, College of Animal Science and Technology & College of Veterinary Medicine, Zhejiang A&F University, Hangzhou, Zhejiang, China
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ZHOU Xiujuan
ZHOU Xiujuan
Key Laboratory of Applied Technology on Green-Eco-Healthy Animal Husbandry of Zhejiang Province, Zhejiang Provincial Engineering Laboratory for Animal Health Inspection & Internet Technology, College of Animal Science and Technology & College of Veterinary Medicine, Zhejiang A&F University, Hangzhou, Zhejiang, China
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ZHONG Xiaojun
ZHONG Xiaojun
Key Laboratory of Applied Technology on Green-Eco-Healthy Animal Husbandry of Zhejiang Province, Zhejiang Provincial Engineering Laboratory for Animal Health Inspection & Internet Technology, College of Animal Science and Technology & College of Veterinary Medicine, Zhejiang A&F University, Hangzhou, Zhejiang, China
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YANG Menghua
YANG Menghua
Key Laboratory of Applied Technology on Green-Eco-Healthy Animal Husbandry of Zhejiang Province, Zhejiang Provincial Engineering Laboratory for Animal Health Inspection & Internet Technology, College of Animal Science and Technology & College of Veterinary Medicine, Zhejiang A&F University, Hangzhou, Zhejiang, China
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Affiliation:

Key Laboratory of Applied Technology on Green-Eco-Healthy Animal Husbandry of Zhejiang Province, Zhejiang Provincial Engineering Laboratory for Animal Health Inspection & Internet Technology, College of Animal Science and Technology & College of Veterinary Medicine, Zhejiang A&F University, Hangzhou, Zhejiang, China

Fund Project:

This work was supported by the National Natural Science Foundation of China (32170174, 32202804), the Natural Science Foundation of Zhejiang Province (LQ22C180002), and the Science Development Foundation of Zhejiang A&F University (2013FR012, 2020FR042).

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摘要:

目的探究组氨酸激酶EnvZ调控副溶血弧菌群集性爬动和生物被膜形成的作用机制。方法利用含有诱导型启动子的pBAD24与pMal质粒，构建相应基因的过表达质粒，并将其导入野生株和envZ基因缺失株中，通过运动性培养基比较各菌株的群集性爬动能力，采用结晶紫染色法检测各菌株的生物被膜形成能力，并结合RT-qPCR与荧光报告系统检测下游基因的表达水平，以探究EnvZ调节副溶血弧菌群集性爬动和生物被膜形成的分子机制。结果 ΔenvZ菌株的群集性爬动能力显著低于野生株，而导入pBAD24-envZ回补质粒的ΔenvZ菌株能够恢复其群集性爬动能力。这些菌株的群集性爬动能力与侧生鞭毛相关基因的表达水平呈正相关。在envZ基因缺失的菌株中，Scr系统启动子的转录活性显著低于野生株和ΔompR菌株。在envZ基因缺失的菌株中过表达Scr系统，可以显著恢复其群集性爬动；然而，在scrABC基因缺失的菌株中过表达EnvZ，并不能改变其群集性爬动能力。ΔenvZ菌株的生物被膜形成能力显著低于野生株，而pMal-envZ质粒能够使ΔenvZ菌株的生物被膜厚度恢复至野生株水平，但pMal-scrABC重组质粒则无此功能。在ΔenvZ菌株中，胞外多糖操纵子(epsA-J)的启动子活性与关键基因的转录水平均显著低于野生株。结论组氨酸激酶EnvZ可通过调控Scr系统的表达来增强副溶血弧菌的群集性爬动能力，同时也可通过调控胞外多糖的表达来促进该菌的生物被膜形成。

关键词:副溶血弧菌;组氨酸激酶;EnvZ/OmpR;群集性爬动;生物被膜

Abstract:

Objective Vibrio parahaemolyticus is a major foodborne pathogen that causes acute gastroenteritis in humans. Here, we aim to decipher the mechanisms by which the histidine kinase EnvZ regulates the swarming motility and biofilm formation of V. parahaemolyticus.Methods The plasmids pBAD24 and pMal carrying inducible promoters were used to construct the plasmids carrying target genes for overexpression. The recombinant plasmids were introduced into the wild-type strain (WT) and envZ-deleted strain (ΔenvZ) of V. parahaemolyticus. Swarming plates were prepared to measure swarming motility, while biofilm formation was detected by crystal violet staining. The RT-qPCR and bioluminescence reporter assays were employed to explore the mechanisms by which EnvZ regulated the expression of downstream genes.Results The swarming motility of ΔenvZ was significantly lower than that of WT, while the introduction of the pBAD24-envZ plasmid into ΔenvZ restored its swarming ability. The transcription levels of the lateral flagellar genes were positively correlated with the swarming motility. The promoter activities of P_scrABC-lux in ΔenvZ and ΔenvZΔompR were lower than those in WT and ΔompR. The swarming ability of ΔenvZ was significantly increased when the Scr system was overexpressed via the pMal-scrABC plasmid, while the overexpression of EnvZ in the strain without scrABC did not change the swarming motility. In addition, ΔenvZ exhibited a significant decrease in biofilm formation compared with WT. The pMal-envZ plasmid restored the biofilm formation of ΔenvZ to the level of WT, whereas the pMal-scrABC plasmid did not have this effect. The promoter activity of the extracellular polysaccharide operon (epsA-J) and the transcription levels of the extracellular polysaccharide genes in ΔenvZ were both significantly lower than those in WT.Conclusion The histidine kinase EnvZ enhances the swarming motility of V. parahaemolyticus by regulating the expression of the Scr system and promotes the biofilm formation by regulating the expression of extracellular polysaccharides.

Key words:Vibrio parahaemolyticus;histidine kinase;EnvZ/OmpR;swarming motility;biofilm

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袁艺萱,吴文婷,陆倩,姚宁,周秀娟,钟孝俊,杨梦华. 组氨酸激酶EnvZ调节副溶血弧菌群集性爬动和生物被膜形成的作用机制[J]. 微生物学报, 2025, 65(5): 2049-2060

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收稿日期:2024-11-06
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