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作 者:黄建斌[1] 王江海[1] 华征[1] 粟文英 宋鸿遇[1]
机构地区:[1]中国科学院上海植物生理研究所
出 处:《植物生理学报(0257-4829)》1996年第2期184-190,共7页Acta Phytophysiologica Sinica
摘 要:紫云英根瘤菌菌株107经Tn5插入诱变,得到12株胞外多糖缺陷型变种,以质粒pMN2为载体,从其中7株EPS-变种内分别构建了7个R-Prime质粒(exoR'),大部分变种的EPS-表型可被exoR'互补,恢复野生型表型(EPS+)。互补表明,12株EPS-变种可分为6个不同的互补群,其中5个在遗传上连锁。exoR'酶切分析,除exoR'-02,exoR'-04外,其余5只的外源片段均整合于PMN2的两同向重复序列IS21之间。Twelve exopolysaccharide (EPS ) deficient (Exo-) mutants were isolatedafter Rhizobium astragalus strain 107 wassubjected to transposon Tn5 mutagenesis. Using the broad host range vectorplasmid PMN2, a kanamycin-sensitivederivative of plasmid R68. 45, we isolated seven R-primes (exoR' )from seven EPS- mutunts of Rhizobium astragalus strain 107. Each exoR'plasmid carrieda specific Tn5 insertion site and itsflanking fragment coding for exopolysaccharide synthesis (Fig. 1 ).When these exoR' plasmids were introduced back into the twelve mutunts, exoR' plasmids were able to complementthe EPS- phenotype of most mutants(Table 1 ). Based on complementationanalysis, twelve EPS mutunts wereclassified into six distinct complementution groups (Fig. 2). Five of the six exoloci were genetically linked. By restriction enzyme analysis, it was shown thatin all exoR' plasmids but exoR'-02 andexoR'-4, the foreign DNA fragmentswere integrated between the tandem rePeat sequence IS21 (Fig. 1 ). The mobilization of megaplasmid and Southernhybridization experiments showed thatthe probeexactly hybridized the toealDNA of these strains with the pRa107b(Fig. 3). It means that the five linkedexo loci were located on the megaplasmid pRa 1 07b.
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