Isolation and characterization of enhanced fluorescence mutants of Rhodopseudomonas capsulata
- 1 May 1983
- journal article
- research article
- Published by American Society for Microbiology in Journal of Bacteriology
- Vol. 154 (2) , 748-755
- https://doi.org/10.1128/jb.154.2.748-755.1983
Abstract
After enrichment by a tetracycline suicide under conditions nonpermissive for the growth of mutants defective in photosynthesis, colonies were-screened for enhanced fluorescence in near-IR light by using high-speed IR photography. Twenty mutants were isolated and the chromatophore membranes were analyzed by a new, rapid microprocedure that revealed many different phenotypes among the mutants. The enhanced fluorescence mutants typically possessed a functional light-harvesting II antenna, but showed reduced or absent light-harvesting I. Twelve isolates were also defective in reaction center polypeptides. An R-prime plasmid that bears 50 kilobases of R. capsulata DNA coding for components of the photosynthetic apparatus, pRPS404, complemented all 20 enhanced fluorescence mutants as demonstrated by the quenching of fluorescence in mutants that had received the R-prime plasmid by conjugation. Fluorescence was regained upon loss of the 50-kilobase insert. Complementation of the fluorescent lesions implies that most or all of the genes necessary for the expression of the reaction center and the light-harvesting antennae are carried by the R-prime plasmid, and that these genes are actively transcribed in the homologous organism. All 20 mutants are complemented by 1 of 2 pBR322 subclones of the R-prime plasmid, pRPSEB2 or pRPSE2. pRPSEB2 bears a 4.5-kilobase fragment of R. capsulata DNA including the rxcA locus and pRPSE2 is a pBR322 derivative bearing a 7.5-kilobase R. capsulata DNA fragment bearing the rxcB locus. These fragments carry sequences necessary for the normal synthesis of the light-harvesting and reaction center polypeptide complexes.This publication has 10 references indexed in Scilit:
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