Micro-homology intermediates: RecA’s transient sampling revealed at the single molecule level

Author:

Lee Andrew J1ORCID,Endo Masayuki2ORCID,Hobbs Jamie K3,Davies A Giles1,Wälti Christoph1

Affiliation:

1. Bioelectronics, The Pollard Institute, School of Electronic and Electrical Engineering, University of Leeds, Woodhouse lane, Leeds LS2 9JT, UK

2. Institute for Integrated Cell-Material Sciences, Kyoto University, Yoshida-ushinomiyacho, Sakyo-ku, Kyoto 606-8501, Japan

3. Department of Physics and Astronomy, University of Sheffield, Houndsfield Road, Sheffield S3 7RH, UK

Abstract

Abstract Recombinase A (RecA) is central to homologous recombination. However, despite significant advances, the mechanism with which RecA is able to orchestrate a search for homology remains elusive. DNA nanostructure-augmented high-speed AFM offers the spatial and temporal resolutions required to study the RecA recombination mechanism directly and at the single molecule level. We present the direct in situ observation of RecA-orchestrated alignment of homologous DNA strands to form a stable recombination product within a supporting DNA nanostructure. We show the existence of subtle and short-lived states in the interaction landscape, which suggests that RecA transiently samples micro-homology at the single RecA monomer-level throughout the search for sequence alignment. These transient interactions form the early steps in the search for sequence homology, prior to the formation of stable pairings at >8 nucleotide seeds. The removal of sequence micro-homology results in the loss of the associated transient sampling at that location.

Funder

Engineering and Physical Sciences Research Council

University of Leeds

Publisher

Oxford University Press (OUP)

Subject

Genetics

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