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Effect of I-SceI Endonuclease on Coincidence of Secondary Mutations with Lac+ Point Mutations.

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Figshare2015-12-02 更新2026-05-11 收录
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aIn this and all of the tables and figures in this paper, stress-induced Lac+ colonies were divided into point mutants (compensatory frameshift revertants) and lac-amplified clones per [14], and only the point mutants were screened for secondary mutations. Because stress-induced lac-amplifications are not associated with secondary mutations (or a HMS) [14], this controls for differential effects of any of the treatments studied on point mutagenesis and amplification.bStrain SMR6277. This strain is a negative control that expresses neither I-SceI endonuclease nor carries the I-SceI cutsite, and so does not make I-SceI-mediated DNA double-strand breaks (DSBs). It is a negative control for the ��Enzyme and Cutsite�� strain SMR6280 which expresses I-SceI from a chromosomal regulatable promoter PBAD replacing the phage lambda attachment site (��att��::PBADI-SceI) and carries an I-SceI site, and makes DSBs. This strain has the PBAD promoter insertion without the I-SceI gene, ��att��::PBAD, and so is designated ��PBAD only��).cStrain SMR6276. This strain is a second negative control for the I-SceI-mediated DSB-producing strain SMR6280. This ��Enzyme-only�� strain carries the ��att��::PBADI-SceI expression cassette but no I-SceI cutsite.dStrain SMR6280, with both the chromosomal ��att��::PBADI-SceI expression cassette and the F'-located I-SceI cutsite, makes I-SceI-induced DSBs near lac[19]. This strain shows greatly increased Lac+ stress-induced mutagenesis ([19] and shown here, Figure 3).e��Mucoid�� colonies had a mucoid appearance on minimal M9 glucose plates and did not form colonies on either maltose or xylose MacConkey medium.
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2015-12-02
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