Isolation of Rhizobium loti Strain-Specific DNA Sequences by Subtraction Hybridization

Author:

Bjourson A. J.1,Cooper J. E.1

Affiliation:

1. Food and Agricultural Microbiology Research Division, Department of Agriculture for Northern Ireland, and The Queen's University of Belfast, 2 Newforge Lane, Belfast BT9 5PX, Northern Ireland

Abstract

Mixed-phase (heterogeneous) and single-phase (homogeneous) DNA subtraction-hybridization methods were used to isolate specific DNA probes for closely related Rhizobium loti strains. In the heterogeneous method, DNA from the prospective probe strain was repeatedly hybridized to a mixture of DNA from cross-hybridizing strains (subtracter DNA) which was immobilized on an epoxy-activated cellulose matrix. Probe strain sequences which shared homology with the matrix-bound subtracter DNA hybridized to it, leaving unique probe strain sequences in the mobile phase. In the homogeneous method, probe strain sequences were hybridized in solution to biotinylated, mercurated subtracter DNA. Biotinylated, mercurated subtracer DNA and probe strain sequences hybridized to it were removed by two-step affinity chromatography on streptavidin-agarose and thiol-Sepharose. The specificity of the sequences remaining after subtraction hybridization by both methods was assessed and compared by colony hybridization with R. loti strains. Both methods allowed the rapid isolation of strain-specific DNA fragments which were suitable for use as probes.

Publisher

American Society for Microbiology

Subject

Ecology,Applied Microbiology and Biotechnology,Food Science,Biotechnology

Reference10 articles.

1. Arrand J. E. 1985. Preparation of nucleic acid probes p. 36-38. In B. D. Hames and S. J. Higgins (ed.) Nucleic acid hybridization. IRL Press Oxford.

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4. Mercurated polynucleotides: new probes for hybridization and selective polymer fractionation;Dale R. M. K.;Biochemistry,1975

5. DNA colony hybridization to identify Rhizobium strains;Hodgson A. L. M.;J. Gen. Microbiol.,1983

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