Analysis of recombination occurring at SLP1 att sites

Lee, S C; Omer, Charles A.; Brasch, Michael A.; Cohen, Stanley N.

doi:10.1128/jb.170.12.5806-5813.1988

Cited by 22 publications

(10 citation statements)

References 33 publications

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“…Sedlmeier and collaborators (204) proposed that the lack of tRNA genes with rRNA genes might be characteristic for all actinomycetes. Based on the first reports that initiator tRNAs from Streptomyces griseus and S. rimosus lack CCA ends (74, 128) and on later publications indicating that potential tRNA Pro , tRNA Thr , and tRNA Tyr genes associated with site-specific recombination in Streptomyces also lack CCA termini (132,143,197), Plohl and Gamulin (185) predicted that most, if not all, tRNA genes in S. rimosus do not encode a CCA terminus. At present, this prediction is still valid and in agreement with current analyses of the tRNA genes based on genome sequencing data.…”

Section: Trna Rrna and Gene Expression In S Rimosusmentioning

confidence: 99%

Genetics ofStreptomyces rimosus, the Oxytetracycline Producer

Petković

Cullum

Hranueli

et al. 2006

Microbiol Mol Biol Rev

101

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SUMMARY From a genetic standpoint, Streptomyces rimosus is arguably the best-characterized industrial streptomycete as the producer of oxytetracycline and other tetracycline antibiotics. Although resistance to these antibiotics has reduced their clinical use in recent years, tetracyclines have an increasing role in the treatment of emerging infections and noninfective diseases. Procedures for in vivo and in vitro genetic manipulations in S. rimosus have been developed since the 1950s and applied to study the genetic instability of S. rimosus strains and for the molecular cloning and characterization of genes involved in oxytetracycline biosynthesis. Recent advances in the methodology of genome sequencing bring the realistic prospect of obtaining the genome sequence of S. rimosus in the near term.

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Section: Trna Rrna and Gene Expression In S Rimosusmentioning

confidence: 99%

Genetics ofStreptomyces rimosus, the Oxytetracycline Producer

Petković

Cullum

Hranueli

et al. 2006

Microbiol Mol Biol Rev

101

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“…Similar experiments reported previously (18) failed to detect these free circular molecules in nonmating cells, leading to the conclusion that excision is induced by mating. While we found a 2-to 10-fold increase in the abundance of autonomous xis+ SLP1 molecules during mating, the presence of precisely excised SLP1 plasmids in nonmating cells indicates that mating is not required for excision.…”

Section: Discussionmentioning

confidence: 57%

“…It is now clear that because the attB site lies within the 3' end of a gene encoding a tRNAT3" essential for viability of S. lividans (29), at least part of the 112-bp homology is required to regenerate this gene upon integration. We have shown previously that no more than 48 bp of the 112-bp attB-attP homology is required for a sequence to function as an attB site (18). However, during construction of a substrate for excision assays, we found that, while the Int-expressing plasmid pSUM307 can promote integration of a plasmid that contains a 485-bp segment of SLP1 DNA flanking attP (pSUM317, Fig.…”

Section: Discussionmentioning

confidence: 71%

Excisive recombination of the SLP1 element in Streptomyces lividans is mediated by Int and enhanced by Xis

Brasch

Cohen

1993

J Bacteriol

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The functions mediating site-specific recombination of the SLP1 element have been mapped to a 2.2-kb region that includes the site of integration (attP), a gene (int) that specifies a function both necessary and sufficient for integration of SLP1, and an open reading frame, orf61, suspected of encoding a protein, Xis, that shows limited similarity to the excisionases of other site-specific recombination systems. Here we describe experiments that investigate the respective roles of or16 and int in the excision of SLP1. We constructed derivatives of the high-copy-number Streptomyces plasmid pU101 that express ori6, int, or both orf6 and int from transcriptional fusions to the TnS aph gene and tested the ability of these constructs to promote excision of an adventitious attP-containing plasmid that had been integrated site-specifically into the atiB site of the Streptomyces lividans chromosome. Expression of the int gene product alone from an exogenous promoter was sufficient for excision of the integrated plasmid. This result indicates that the SLP1 int-encoded protein can carry out excisive, as well as integrative, recombination. The orf6l gene product, when expressed from an exogenous promoter, inhibited int-mediated integration at the chromosomal atB site. Moreover, under conditions in which excision and transfer normally occur, precise excision of SLP1 was enhanced by the or61-encoded protein. On the basis of these findings, we here designate the or61 gene as xis.SLP1, a 17.2-kbp DNA segment indigenous to the chromosome of Streptomyces coelicolor, is the prototype of a family of transmissible chromosomally integrating plasmidogenic genetic elements of the actinomyces (reviewed in references 1, 2, and 23). In the accompanying report (7), we demonstrate that a 2.2-kb segment of SLP1 contains all of the functions required for site-specific integration of SLP1 into the Streptomyces lividans chromosome. Nucleotide sequence analysis of this DNA revealed two open reading frames, one of which encodes a putative 50.5-kDa protein having substantial similarity to a family of site-specific recombinases that includes the Escherichia coli bacteriophage X integrase. The product of this open reading frame was shown to be both necessary and sufficient for integration of SLP1 in S. lividans and accordingly has been designated as the Int protein. The second open reading frame, orf6l, which lies immediately 5' to int, corresponds to a 61-aminoacid basic peptide showing limited similarity to the excisionase (xis) gene products of other site-specific recombination systems.In other recombination systems that encode proteins resembling the int and orf6l gene products, integration requires, in addition to host factors, only integrase, whereas excision ordinarily requires both integrase and an excisionase protein (1,2,14,19). We report here the results of studies that analyze the respective roles of the SLP1 int and orf6l genes in excisive recombination. We find that, under conditions in which the integrase is expressed under the contr...

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“…For example, a cross in which S. coelicolor A3(2) served as the donor and S. lividans 66 functioned as the recipient revealed the presence of a 17-kb plasmidogenic locus in the former (258). Upon transfer, the locus could exist in the recipient in three forms: transiently as a 17-kb plasmid containing all the genetic content present in the original locus, integrated at a specific site in the S. lividans chromosome (203,259,260), or as one of several smaller plasmids, 11 to 14.5 kb in size (153). In the smaller plasmids, genetic information for integration and maintenance was deleted.…”

Section: Effective Abundance Of Gene Copiesmentioning

confidence: 99%

Organization of the Bacterial Chromosome

Schumann

2006

Dynamics of the Bacterial Chromosome

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Analysis of recombination occurring at SLP1 att sites

Cited by 22 publications

References 33 publications

Genetics ofStreptomyces rimosus, the Oxytetracycline Producer

Genetics ofStreptomyces rimosus, the Oxytetracycline Producer

Excisive recombination of the SLP1 element in Streptomyces lividans is mediated by Int and enhanced by Xis

Organization of the Bacterial Chromosome

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