农业科学与技术:英文版
農業科學與技術:英文版
농업과학여기술:영문판
Agricultural Science & Technology
2012年
3期
492-496
,共5页
王青柏%胡超群%陈偿%徐鹏
王青柏%鬍超群%陳償%徐鵬
왕청백%호초군%진상%서붕
溶藻弧菌%vsc基因%自杀质粒%同源重组
溶藻弧菌%vsc基因%自殺質粒%同源重組
용조호균%vsc기인%자살질립%동원중조
Vibrio alginolyticus%vscC gene%Suicide plasmid%Homologous recombination
[目的]构建未引入任何遗传标记物的溶藻弧菌vscC基因框内缺失突变株。[方法]首先以溶藻弧菌ZJ51-O基因组DNA为模板,用重叠延伸PCR(gene splicing by overlap extension PCR,SOE-PCR)扩增法构建体外vscC基因缺失片段;扩增产物经酶切后连接至自杀质粒pDM4,再转化入大肠杆菌SY327进行克隆,筛选阳性克隆子并进行PCR分析鉴定;提取阳性克隆子的自杀重组质粒pDM4-/△vscC,用热休克法将其转入到大肠杆菌s17—1中,再经接合生殖的方式将自杀重组质粒导入溶藻弧菌ZJ51-0菌株中,利用抗生素筛选策略与蔗糖反向筛选系统,挑选疑似目的突变菌株,最后利用PCR鉴定与测序分析进行确证。[结果]溶藻弧菌ZJ51-O的vscC基因框内缺失突变株构建成功。[结论]该研究为进一步研究vscC基因的功能和T3SS在溶藻弧菌致病过程中所起的作用奠定基础,同时也为溶藻弧菌的其他基因突变株的构建和研究提供了参考和试验经验。
[目的]構建未引入任何遺傳標記物的溶藻弧菌vscC基因框內缺失突變株。[方法]首先以溶藻弧菌ZJ51-O基因組DNA為模闆,用重疊延伸PCR(gene splicing by overlap extension PCR,SOE-PCR)擴增法構建體外vscC基因缺失片段;擴增產物經酶切後連接至自殺質粒pDM4,再轉化入大腸桿菌SY327進行剋隆,篩選暘性剋隆子併進行PCR分析鑒定;提取暘性剋隆子的自殺重組質粒pDM4-/△vscC,用熱休剋法將其轉入到大腸桿菌s17—1中,再經接閤生殖的方式將自殺重組質粒導入溶藻弧菌ZJ51-0菌株中,利用抗生素篩選策略與蔗糖反嚮篩選繫統,挑選疑似目的突變菌株,最後利用PCR鑒定與測序分析進行確證。[結果]溶藻弧菌ZJ51-O的vscC基因框內缺失突變株構建成功。[結論]該研究為進一步研究vscC基因的功能和T3SS在溶藻弧菌緻病過程中所起的作用奠定基礎,同時也為溶藻弧菌的其他基因突變株的構建和研究提供瞭參攷和試驗經驗。
[목적]구건미인입임하유전표기물적용조호균vscC기인광내결실돌변주。[방법]수선이용조호균ZJ51-O기인조DNA위모판,용중첩연신PCR(gene splicing by overlap extension PCR,SOE-PCR)확증법구건체외vscC기인결실편단;확증산물경매절후련접지자살질립pDM4,재전화입대장간균SY327진행극륭,사선양성극륭자병진행PCR분석감정;제취양성극륭자적자살중조질립pDM4-/△vscC,용열휴극법장기전입도대장간균s17—1중,재경접합생식적방식장자살중조질립도입용조호균ZJ51-0균주중,이용항생소사선책략여자당반향사선계통,도선의사목적돌변균주,최후이용PCR감정여측서분석진행학증。[결과]용조호균ZJ51-O적vscC기인광내결실돌변주구건성공。[결론]해연구위진일보연구vscC기인적공능화T3SS재용조호균치병과정중소기적작용전정기출,동시야위용조호균적기타기인돌변주적구건화연구제공료삼고화시험경험。
[Objective] The purpose of this study was to construct a vscC in-frame deletion mutant of Vibrio alginolyticus with no antibiotic resistance marker. [Method] The first vscC mutant molecules in vitro were generated by SOE-PCR and then lig- ated to a suicide vector pDM4 to construct a suicide recombinant vector pDM4- A vscC. To clone the recombinant vector, it was transformed to E. coli SY327 strain, and then positive clones were selected and proved by PCR analysis. After that, the pDM4-AvscC DNA was extracted in large numbers and transformed to the E. coil S17-1 strain that acted as a donor in bacterial conjugation using the heat shock method. The recombinant E. coli S17-1 strains then transferred the pDM4-AvscC to V. alginolyticus ZJ51-O by conjugation method; transconjugants were screened and selected sequentially using antibiotic selection strategy and sucrose based counter-selection system to find the suspected mutants wanted. Finally the putative mutants were identified by PCR and confirmed by sequencing analysis. [Result] ZJ51-OAvscC was successfully constructed. [Conclusion] This study laid foundation for further research on the function of vscC gene and molecular mechanism of type Ⅲ secretion system in V. alginolyticus. Simultaneously, by the effective method other unknown functional genes in V. alginolyticus genome would be researched.
