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Integron integrase binds to bulged hairpin DNA
Uppsala universitet, Medicinska vetenskapsområdet, Medicinska fakulteten, Institutionen för medicinsk biokemi och mikrobiologi.
2004 Ingår i: Nucleic Acids Res, ISSN 0305-1048, Vol. 32, nr 13, s. 4033-4043Artikel i tidskrift (Refereegranskat) Published
Ort, förlag, år, upplaga, sidor
2004. Vol. 32, nr 13, s. 4033-4043
Identifikatorer
URN: urn:nbn:se:uu:diva-95307OAI: oai:DiVA.org:uu-95307DiVA, id: diva2:169474
Tillgänglig från: 2007-01-02 Skapad: 2007-01-02Bibliografiskt granskad
Ingår i avhandling
1. Mechanisms and DNA Specificity in Site-specific Recombination of Integron Cassettes
Öppna denna publikation i ny flik eller fönster >>Mechanisms and DNA Specificity in Site-specific Recombination of Integron Cassettes
2007 (Engelska)Doktorsavhandling, sammanläggning (Övrigt vetenskapligt)
Abstract [en]

Bacterial resistance to antibiotics has become a serious problem. This is due to the remarkable ability of bacteria to respond and rapidly adapt to environmental changes. Integrons are elements with the capacity for gene capture by an integron-encoded site-specific recombinase called IntI. IntI binds and acts at the recombination sites, attI and attC resulting in excision and integration of short DNA elements called gene cassettes carrying an attC site in the 3’ end. Several families of antibiotic resistance genes are borne on gene cassettes in integrons connected to mobile elements. Other cassettes reside in the larger and ancestral superintegrons located on chromosomes in both pathogenic and environmental bacteria. Due to their close connection with lateral gene transfer systems, it is possible that integrons are functionally dependent on those networks. This work presents arguments for such connections. The attC of the aadA1-qacE cassette junction in Tn21 was characterized in detail. Like other attC sites, it contains two pairs of inverted repeats and is almost palindromic. By using electrophoretic mobility shift assays, this study showed that IntI1 binds only to the bottom strand of attC. Upon folding the strand into a hairpin, a few chiral hairpin distortions define both the strand choice and also the appropriate orientation of the highly symmetrical site. Structural recognition also explains the wide sequence variation among attC sites. We have documented the initial cleavage step in recombination in IntI extracts and integrase levels in extracts were evaluated by a new method. Mutagenesis and homology modelling were performed to find amino acid residues in IntI1 that are important for recognition of attC hairpin-DNA. Comparisons were made with other tyrosine family members to explain how integron integrases differ in site-recognition and also in their mechanism of strand exchange.

Ort, förlag, år, upplaga, sidor
Uppsala: Acta Universitatis Upsaliensis, 2007. s. 65
Serie
Digital Comprehensive Summaries of Uppsala Dissertations from the Faculty of Medicine, ISSN 1651-6206 ; 214
Nyckelord
Microbiology, lateral gene transfer, site-specific recombination, tyrosine recombinase, integron, single-stranded, DNA hairpin, Mikrobiologi
Forskningsämne
farmaceutisk mikrobiologi
Identifikatorer
urn:nbn:se:uu:diva-7429 (URN)978-91-554-6767-8 (ISBN)
Disputation
2007-01-24, C10:301, BMC, Husargatan 3, Uppsala, 09:15
Opponent
Handledare
Tillgänglig från: 2007-01-02 Skapad: 2007-01-02Bibliografiskt granskad

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