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鼠伤寒沙门菌yibTcsgD双基因缺失株的构建及对生物膜形成的影响

刘晓彤 王冰冰 王治梅 刘菲凡 赵威 齐永华

刘晓彤,王冰冰,王治梅,等. 鼠伤寒沙门菌yibT和csgD双基因缺失株的构建及对生物膜形成的影响 [J]. 福建农业学报,2024,39(8):879−887 doi: 10.19303/j.issn.1008-0384.2024.08.001
引用本文: 刘晓彤,王冰冰,王治梅,等. 鼠伤寒沙门菌yibTcsgD双基因缺失株的构建及对生物膜形成的影响 [J]. 福建农业学报,2024,39(8):879−887 doi: 10.19303/j.issn.1008-0384.2024.08.001
LIU X T, WANG B B, WANG Z M, et al. Construction and Biofilm Formation of yibT-and-csgD-deleted Salmonella typhimurium [J]. Fujian Journal of Agricultural Sciences,2024,39(8):879−887 doi: 10.19303/j.issn.1008-0384.2024.08.001
Citation: LIU X T, WANG B B, WANG Z M, et al. Construction and Biofilm Formation of yibT-and-csgD-deleted Salmonella typhimurium [J]. Fujian Journal of Agricultural Sciences,2024,39(8):879−887 doi: 10.19303/j.issn.1008-0384.2024.08.001

鼠伤寒沙门菌yibTcsgD双基因缺失株的构建及对生物膜形成的影响

doi: 10.19303/j.issn.1008-0384.2024.08.001
基金项目: 河南省自然科学基金项目(222300420510)
详细信息
    作者简介:

    刘晓彤(1999—),女,硕士研究生,主要从事兽医药理学相关研究,E-mail:1036144263@qq.com

    通讯作者:

    齐永华(1977—),男,博士,教授,主要从事病原微生物控制及新药研发相关研究, E-mail:qyh@xxu.edu.cn

  • 中图分类号: S852

Construction and Biofilm Formation of yibT-and-csgD-deleted Salmonella typhimurium

  • 摘要:   目的  通过构建鼠伤寒沙门菌(Salmonella typhimuriumyibTcsgD双基因缺失株及缺失株的回补株,探究其对鼠伤寒沙门菌生物膜形成的影响,以期为沙门菌的有效防控提供新策略。  方法  以鼠伤寒沙门菌野生株CVCC541(wild-type, WT)为研究对象,利用λ-red同源重组技术构建yibTcsgD基因缺失株;利用重组载体技术构建其基因回补株;利用结晶紫染色法比较鼠伤寒沙门菌突变株生物膜形成能力的差异;通过苯酚-硫酸法测定胞外多糖含量、半固体平板测定运动能力的变化;比较不同突变菌株自聚集能力的变化;通过扫描电镜观察生物膜结构;最后利用荧光定量PCR技术鉴定生物膜形成过程中关键基因的mRNA表达水平。  结果  成功构建了鼠伤寒沙门菌yibTcsgD的双基因缺失株WTΔyibTΔcsgD和csgD基因单缺失株WTΔcsgD及基因缺失株的回补株WTΔcsgDΔyibT/pcsgD和WTΔcsgD/pcsgD。 yibTcsgD基因的缺失降低了生物膜的形成能力、胞外多糖含量和自聚集能力,增强了运动能力;invFsdiA基因的mRNA表达水平下降。  结论  yibTcsgD基因缺失会降低鼠伤寒沙门菌的生物膜形成能力。
  • 图  1  菌株WTΔyibTΔcsgD:Kan和WTΔcsgD:Kan的PCR鉴定

    M:D2000 Marker;1:WTΔyibTΔcsgD:Kan PCR产物;2: WTΔcsgD:Kan PCR产物;3:WT PCR产物。

    Figure  1.  PCR identification for WTΔyibTΔcsgD:Kan and WTΔcsgD:Kan

    M: D2000 marker; 1: PCR product of WTΔyibTΔcsgD:Kan; 2: PCR product of WTΔcsgD:Kan; 3: PCR product of WT.

    图  2  菌株WTΔyibTΔcsgD和WTΔcsgD的PCR鉴定

    M:D2000 Marker;1:WT 的 PCR 产物;2:WTΔyibTΔcsgD 的 PCR 产物;3:WTΔcsgD 的 PCR 产物。

    Figure  2.  PCR identification for WTΔyibTΔcsgD and WTΔcsgD

    M: D2000 marker; 1: PCR product of WT; 2: PCR product of WTΔyibTΔcsgD; 3: PCR product of WTΔcsgD.

    图  3  WTΔyibTΔcsgD/pcsgD和WTΔcsgD/pcsgD的PCR鉴定

    M:D2000 Marker;1:WTΔyibTΔcsgD/pcsgD的PCR产物;2:WTΔcsgD/pcsgD的PCR产物;3:转入空质粒pET28a的菌 PCR产物。

    Figure  3.  PCR identification for WTΔyibTΔcsgD/pcsgD and WTΔcsgD/pcsgD

    M: D2000 marker; 1: PCR product of WTΔyibTΔcsgD/pcsgD; 2: PCR product of WTΔcsgD/pcsgD; 3: PCR product of bacteria transferred to empty plasmid pET28a.

    图  4  鼠伤寒沙门菌突变株的生物膜形成

    A:试管法测定生物膜能力;B:二十四孔板测定生物膜能力;C:生物膜的结晶紫量化。*表示与WT差异显著(P<0.05),**表示与WT差异极显著(P<0.01)。下同。

    Figure  4.  Biofilm formation of S. typhimurium mutants

    A: test tube method for determining biofilm formation; B: 24-well plates for determining biofilm formation; C: crystal violet quantization of biofilm. Results are comparisons with WT; *: significant difference at P<0.05; **: extremely significant difference at P<0.01. Same for below.

    图  5  鼠伤寒沙门菌突变株的生物膜结构

    Figure  5.  Biofilm structure of S. typhimurium mutants

    图  6  鼠伤寒沙门菌突变株胞外多糖含量

    A:葡萄糖标准曲线;B:胞外多糖含量。

    Figure  6.  Exopolysaccharide contents in S. typhimurium mutants

    A: glucose standard curve; B: exopolysaccharide content.

    图  7  鼠伤寒沙门菌突变株的运动能力

    A:鼠伤寒沙门菌突变株在半固体平板的运动性;B:鼠伤寒沙门菌突变株的运动直径。

    Figure  7.  Motility of S. typhimurium mutants

    A: motility of S. typhimurium mutants on semi-solid plates; B: diameters of moving area of S. typhimurium mutants.

    图  8  鼠伤寒沙门菌突变株的自聚集情况

    Figure  8.  Self-aggregation of S. typhimurium mutants

    图  9  鼠伤寒沙门菌突变株的mRNA的表达水平

    Figure  9.  mRNA expressions of S. typhimurium mutants

    表  1  PCR扩增引物

    Table  1.   Primers applied for PCR

    引物名称
    Primer names
    引物序列5′-3′
    Primer sequences
    引物长度
    Primer length/bp
    反应长度
    Reaction length/bp
    P1 TTTCATCATGTTTAATGAAGTCCATAGTAGTCATGGTCAGTGTAGGCTGGAGCTGCTTC 59 1600
    P2 ATCTTTTTGAAAAGATTATAAAGATGTGTCTTAACCGTACATATGAATATCCTCCTTAG 59
    P3 GCTGTCAGATGTGCGATT 18 723
    P4 TGCTACAATCCAGGTCAGA 19
    P5 CCGCTCGAGCCGCCTGAGATTATCGTTTG 29 649
    P6 CGCGGATCCATGTTTAATGAAGTCCATAG 29
    P7 CAGCCAGGCGTTCCGTGAAT 20 469
    P8 AGCCGCCGGTAATATTCCAGAC 22
    下载: 导出CSV

    表  2  荧光定量PCR引物序列

    Table  2.   Primers applied for qRT-PCR

    引物名称
    Primer names
    引物序列5′-3′
    Primer sequences
    引物长度
    Primer length/bp
    luxS-F ACTGATGGGCTGCCTGTATC 20
    luxS-R
    sdiA-F
    sdiA-R
    invF-F
    invF-R
    16S-F
    16S-R
    GCCTCTTCGCTATTACGCCA
    ATGAAGCGAAGGCGATGT
    CGAGGAGCAGCGTAAACT
    ACGATGAGAATGCTGGGAGA
    TATGTGAAGGCGATGAGTAAC
    TTACCCGCAGAAGAAGCACC
    CTCAAGGGCACAACCTCCAA
    20
    18
    18
    20
    20
    20
    20
    下载: 导出CSV
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出版历程
  • 收稿日期:  2024-05-13
  • 修回日期:  2024-08-04
  • 网络出版日期:  2024-11-13
  • 刊出日期:  2024-08-28

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