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Multiple serine transposase dimers assemble the transposon-end synaptic complex during IS607-family transposition.


ABSTRACT: IS607-family transposons are unusual because they do not have terminal inverted repeats or generate target site duplications. They encode two protein-coding genes, but only tnpA is required for transposition. Our X-ray structures confirm that TnpA is a member of the serine recombinase (SR) family, but the chemically-inactive quaternary structure of the dimer, along with the N-terminal location of the DNA binding domain, are different from other SRs. TnpA dimers from IS1535 cooperatively associate with multiple subterminal repeats, which together with additional nonspecific binding, form a nucleoprotein filament on one transposon end that efficiently captures a second unbound end to generate the paired-end complex (PEC). Formation of the PEC does not require a change in the dimeric structure of the catalytic domain, but remodeling of the C-terminal ?-helical region is involved. We posit that the PEC recruits a chemically-active conformer of TnpA to the transposon end to initiate DNA chemistry.

SUBMITTER: Chen W 

PROVIDER: S-EPMC6188088 | biostudies-literature | 2018 Oct

REPOSITORIES: biostudies-literature

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Multiple serine transposase dimers assemble the transposon-end synaptic complex during IS<i>607</i>-family transposition.

Chen Wenyang W   Chen Wenyang W   Mandali Sridhar S   Hancock Stephen P SP   Kumar Pramod P   Collazo Michael M   Cascio Duilio D   Johnson Reid C RC  

eLife 20181005


IS<i>607</i>-family transposons are unusual because they do not have terminal inverted repeats or generate target site duplications. They encode two protein-coding genes, but only <i>tnpA</i> is required for transposition. Our X-ray structures confirm that TnpA is a member of the serine recombinase (SR) family, but the chemically-inactive quaternary structure of the dimer, along with the N-terminal location of the DNA binding domain, are different from other SRs. TnpA dimers from IS<i>1535</i> c  ...[more]

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