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根癌土壤杆菌Ti质粒pTiC58接合转移功能的表征

Characterization of conjugal transfer functions of Agrobacterium tumefaciens Ti plasmid pTiC58.

作者信息

von Bodman S B, McCutchan J E, Farrand S K

机构信息

Department of Plant Pathology, University of Illinois, Urbana 61801.

出版信息

J Bacteriol. 1989 Oct;171(10):5281-9. doi: 10.1128/jb.171.10.5281-5289.1989.

Abstract

Physical characterization of 13 transposon Tn5 insertions within the agrocinopine-independent, transfer-constitutive Ti plasmid pTiC58Trac identified three separate loci essential for conjugation of this nopaline/agrocinopine A + B-type Ti plasmid. Complementation analysis with relevant subcloned DNAs indicated that the three physically separated blocks of conjugal genes constitute distinct complementation groups. Two independent Tn5 insertions within the wild-type, agrocinopine-dependent, repressed pTiC58 plasmid resulted in constitutive expression of conjugal transfer. These two insertions were physically indistinguishable and could not be complemented in trans. However, the Trac phenotype resulted when the Tn5-mutated fragment cointegrated into the wild-type Ti plasmid. While the spontaneous Trac mutant Ti plasmids were also derepressed for agrocinopine catabolism, those generated by Tn5 insertions remained inducible, indicating that this apparent cis-acting site is different from that affected in the spontaneous mutants. No chromosomal Tn5 insertion mutations were obtained that affected conjugal transfer. An octopine-type Ti plasmid, resident in different Agrobacterium tumefaciens chvB mutants, transferred at normal frequencies, demonstrating that this virulence locus affecting plant cell binding is not required for Ti plasmid conjugation. None of our conjugal mutants limited tumor development on Kalanchoe diagremontiana. Known lesions in pTiC58 vir loci had no effect on conjugal transfer of this Ti plasmid. These results show that pTiC58 Ti plasmid conjugal transfer occurs by functions independent of those required for transfer of DNA to plant cells.

摘要

对农杆碱非依赖型、转移组成型Ti质粒pTiC58Trac上的13个转座子Tn5插入进行物理表征,确定了该胭脂碱/农杆碱A + B型Ti质粒接合所必需的三个独立位点。用相关亚克隆DNA进行互补分析表明,三个物理上分离的接合基因块构成了不同的互补群。野生型、农杆碱依赖型、受抑制的pTiC58质粒中的两个独立Tn5插入导致接合转移的组成型表达。这两个插入在物理上无法区分,并且不能在反式中互补。然而,当Tn5突变片段共整合到野生型Ti质粒中时,产生了Trac表型。虽然自发的Trac突变Ti质粒在农杆碱分解代谢方面也去抑制,但由Tn5插入产生的那些仍然是可诱导的,这表明这个明显的顺式作用位点与自发突变体中受影响的位点不同。没有获得影响接合转移的染色体Tn5插入突变。驻留在不同根癌土壤杆菌chvB突变体中的章鱼碱型Ti质粒以正常频率转移,表明这种影响植物细胞结合的毒力位点对于Ti质粒接合不是必需的。我们的任何接合突变体都没有限制在落地生根上的肿瘤发展。pTiC58 vir位点中的已知损伤对该Ti质粒的接合转移没有影响。这些结果表明,pTiC58 Ti质粒的接合转移是通过独立于将DNA转移到植物细胞所需的功能发生的。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a84b/210363/72ec01740fb3/jbacter00176-0057-a.jpg

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