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菊欧文氏菌中果胶酸裂解酶基因家族的组织方式。

Organization of a pectate lyase gene family in Erwinia chrysanthemi.

作者信息

Reverchon S, Van Gijsegem F, Rouve M, Kotoujansky A, Robert-Baudouy J

出版信息

Gene. 1986;49(2):215-24. doi: 10.1016/0378-1119(86)90282-9.

DOI:10.1016/0378-1119(86)90282-9
PMID:3569916
Abstract

The pelA, pelD and pelE genes encode three of the five major pectate lyase (PL) isoenzymes (PLa, PLd and PLe) in Erwinia chrysanthemi strains B374 and 3937. These genes were previously isolated from genomic libraries or by in vivo cloning as R' factors promoted by the pULB113 plasmid. They are clustered near purE on the chromosomal map of E. chrysanthemi B374 [Van Gijsegem et al., EMBO J. 4 (1985) 787-792]. Genes pelA, pelD and pelE were subcloned separately into pBR322 derivatives, to test their individuality. It then became possible to select specific mutations in each separated gene. Such mutations were obtained using the transposable bacteriophage MudI1734 that allows the construction of lacZ gene fusions. Subcloning experiments and analysis of MudI1734 insertions permitted us to determine the length of each gene, the transcriptional orientation and the location of the promoter. We concluded that the three genes constitute three independent transcriptional units. They are clustered on a 5-kb DNA fragment, in the order: pelD-pelE-pelA. Genes pelD and pelE are transcribed in the same direction, while the transcription of pelA seems to be divergent. Organization of the pel region was very similar in the two strains B374 and 3937. Moreover, lacZ gene fusions were introduced by marker exchange into the chromosome of E. chrysanthemi B374, giving rise to three strains lacking PLa, PLd or PLe. These fusions allowed us to study the regulation of the mutagenized genes.

摘要

在菊欧文氏菌B374和3937菌株中,pelA、pelD和pelE基因编码五种主要果胶酸裂解酶(PL)同工酶中的三种(PLa、PLd和PLe)。这些基因先前是从基因组文库中分离出来的,或者是通过体内克隆,作为由pULB113质粒促进的R'因子分离出来的。它们在菊欧文氏菌B374的染色体图谱上靠近purE基因成簇分布[Van Gijsegem等人,《欧洲分子生物学组织杂志》4(1985)787 - 792]。pelA、pelD和pelE基因分别亚克隆到pBR322衍生物中,以测试它们的独立性。然后就有可能在每个分离的基因中选择特定的突变。使用可转座噬菌体MudI1734获得了这样的突变,该噬菌体允许构建lacZ基因融合体。亚克隆实验和对MudI1734插入的分析使我们能够确定每个基因的长度、转录方向和启动子的位置。我们得出结论,这三个基因构成三个独立的转录单元。它们聚集在一个5 kb的DNA片段上,顺序为:pelD - pelE - pelA。pelD和pelE基因朝同一方向转录,而pelA的转录似乎是相反的。在B374和3937这两个菌株中,pel区域的组织非常相似。此外,通过标记交换将lacZ基因融合体导入菊欧文氏菌B374的染色体,产生了三个缺乏PLa、PLd或PLe的菌株。这些融合体使我们能够研究诱变基因的调控。

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