| Literature DB >> 30787104 |
Yuanlei Cheng1, Qingnan Tang2, Yutong Li1, Yashuo Zhang1, Chuyuan Zhao2, Jie Yan2,3, Huijuan You4.
Abstract
The G-rich Pu39 region of the P1 promoter of the oncogene BCL-2, an apoptosis regulator, can fold into multiple G-quadruplex (G4) structures. Bcl2-2345 and Bcl2-1245 are two major G4 species forming with high thermal stability and distinct topologies in the Pu39 region, but their folding/unfolding kinetics have not yet been investigated. Here, we used magnetic tweezers to measure the mechanical stability and the folding/unfolding kinetics of the Bcl2-2345 and Bcl2-1245 G4 structures. We report that the hybrid-stranded Bcl2-2345 G4 had a lower mechanical stability than the parallel-stranded Bcl2-1245 G4. We observed that the Bcl2-2345 G4 is a kinetically favored structure, whereas the Bcl2-1245 G4, with a slow unfolding rate, may function as a kinetic barrier for transcription. We also determined that in addition to the Bcl2-2345 and Bcl2-1245 G4s, other stable DNA secondary structures, such as a hybrid-stranded Bcl2-1234 G4, can also form in the Pu39 sequence. The characterization of the folding/unfolding kinetics of specific G4s reported here sheds light on the participation of G4s during gene transcription and provides information for designing G4-targeting small molecules that could modulate BCL-2 gene expression.Entities:
Keywords: B-cell lymphoma 2 (Bcl-2); DNA secondary structure; G-quadruplex; folding/unfolding kinetics; force spectroscopy; magnetic tweezers; oncogene promoter; promoter; single-molecule biophysics; transcription regulation
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Year: 2019 PMID: 30787104 PMCID: PMC6463710 DOI: 10.1074/jbc.RA119.007516
Source DB: PubMed Journal: J Biol Chem ISSN: 0021-9258 Impact factor: 5.157