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多氯联苯降解菌的基因构建

Genetic construction of PCB degraders.

作者信息

Brenner V, Arensdorf J J, Focht D D

机构信息

Department of Soil and Environmental Sciences, University of California, Riverside 92521-0424.

出版信息

Biodegradation. 1994 Dec;5(3-4):359-77. doi: 10.1007/BF00696470.

DOI:10.1007/BF00696470
PMID:7765843
Abstract

Genetic construction of recombinant strains with expanded degradative abilities may be useful for bioremedation of recalcitrant compounds, such as polychlorinated biphenyls (PCBs). Some degradative genes have been found either on conjugative plasmids or on transposons, which would facilitate their genetic transfer. The catabolic pathway for the total degradation of PCBs is encoded by two different sets of genes that are not normally found in the same organism. The bphABCD genes normally reside on the chromosome and encode for the four enzymes involved in the production of benzoate and chlorobenzoates from the respective catabolism of biphenyl and chlorobiphenyls. The genes encoding for chlorobenzoate catabolism have been found on both plasmids and the chromosome, often in association with transposable elements. Ring fission of chlorobiphenyls and chlorobenzoates involves the meta-fission pathway (3-phenylcatechol 2,3-dioxygenase) and the ortho-fission pathway (chlorocatechol 1,2-dioxygenase), respectively. As the catecholic intermediates of both pathways are frequently inhibitory to each other, incompatibilities result. Presently, all hybrid strains constructed by in vivo matings metabolize simple chlorobiphenyls through complementary pathways by comprising the bph, benzoate, and chlorocatechol genes of parental strains. No strains have yet been verified which are able to utilize PCBs having at least one chlorine on each ring as growth substrates. The possible incompatibilities of hybrid pathways are evaluated with respect to product toxicity, and the efficiency of both in vivo and in vitro genetic methods for the construction of recombinant strains able to degrade PCBs is discussed.

摘要

构建具有增强降解能力的重组菌株可能有助于对多氯联苯(PCBs)等难降解化合物进行生物修复。一些降解基因已在接合质粒或转座子上被发现,这将便于它们的基因转移。多氯联苯完全降解的分解代谢途径由两组不同的基因编码,而这两组基因通常不存在于同一生物体中。bphABCD基因通常位于染色体上,编码参与从联苯和氯联苯各自的分解代谢中产生苯甲酸和氯苯甲酸的四种酶。编码氯苯甲酸分解代谢的基因已在质粒和染色体上都被发现,并且常常与转座元件相关联。氯联苯和氯苯甲酸的环裂解分别涉及间位裂解途径(3-苯基儿茶酚2,3-双加氧酶)和邻位裂解途径(氯儿茶酚1,2-双加氧酶)。由于这两种途径的儿茶酚中间体常常相互抑制,因此会产生不相容性。目前,通过体内交配构建的所有杂交菌株通过包含亲本菌株的bph、苯甲酸和氯儿茶酚基因,通过互补途径代谢简单的氯联苯。尚未有菌株被证实能够将每个环上至少有一个氯原子的多氯联苯作为生长底物利用。针对产物毒性评估了杂交途径可能存在的不相容性,并讨论了体内和体外构建能够降解多氯联苯的重组菌株的遗传方法的效率。

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