DNA G-Quadruplex Recognition In Vitro and in Live Cells by a Structure-Specific Nanobody
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Galli, Silvia
[1
,2
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Melidis, Larry
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Canc Res UK Cambridge Inst, Cambridge CB2 0RE, England
Univ Cambridge, Yusuf Hamied Dept Chem, Cambridge CB2 1EW, EnglandCanc Res UK Cambridge Inst, Cambridge CB2 0RE, England
Melidis, Larry
[1
,2
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Flynn, Sean M.
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Canc Res UK Cambridge Inst, Cambridge CB2 0RE, EnglandCanc Res UK Cambridge Inst, Cambridge CB2 0RE, England
Flynn, Sean M.
[1
]
Varshney, Dhaval
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Canc Res UK Cambridge Inst, Cambridge CB2 0RE, EnglandCanc Res UK Cambridge Inst, Cambridge CB2 0RE, England
Varshney, Dhaval
[1
]
Simeone, Angela
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Canc Res UK Cambridge Inst, Cambridge CB2 0RE, EnglandCanc Res UK Cambridge Inst, Cambridge CB2 0RE, England
Simeone, Angela
[1
]
Spiegel, Jochen
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Canc Res UK Cambridge Inst, Cambridge CB2 0RE, England
Univ Cambridge, Yusuf Hamied Dept Chem, Cambridge CB2 1EW, EnglandCanc Res UK Cambridge Inst, Cambridge CB2 0RE, England
Spiegel, Jochen
[1
,2
]
Madden, Sarah K.
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Canc Res UK Cambridge Inst, Cambridge CB2 0RE, England
Univ Cambridge, Yusuf Hamied Dept Chem, Cambridge CB2 1EW, EnglandCanc Res UK Cambridge Inst, Cambridge CB2 0RE, England
Madden, Sarah K.
[1
,2
]
Tannahill, David
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Canc Res UK Cambridge Inst, Cambridge CB2 0RE, EnglandCanc Res UK Cambridge Inst, Cambridge CB2 0RE, England
Tannahill, David
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Balasubramanian, Shankar
[1
,2
,3
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[1] Canc Res UK Cambridge Inst, Cambridge CB2 0RE, England
[2] Univ Cambridge, Yusuf Hamied Dept Chem, Cambridge CB2 1EW, England
[3] Univ Cambridge, Sch Clin Med, Cambridge CB2 0SP, England
G-quadruplexes (G4s) are four-stranded DNA secondary structures that occur in the human genome and play key roles in transcription, replication, and genome stability. G4-specific molecular probes are of vital importance to elucidate the structure and function of G4s. The scFv antibody BG4 has been a widely used G4 probe but has various limitations, including relatively poor in vitro expression and the inability to be expressed intracellularly to interrogate G4s in live cells. To address these considerations, we describe herein the development of SG4, a camelid heavy-chain-only derived nanobody that was selected against the human Myc DNA G4 structure. SG4 exhibits low nanomolar affinity for a wide range of folded G4 structures in vitro. We employed AlphaFold combined with molecular dynamics simulations to construct a molecular model for the G4-nanobody interaction. The structural model accurately explains the role of key amino acids and Kd measurements of SG4 mutants, including arginine-to-alanine point mutations that dramatically diminish G4 binding affinity. Importantly, predicted amino acid-G4 interactions were subsequently confirmed experimentally by biophysical measurements. We demonstrate that the nanobody can be expressed intracellularly and used to image endogenous G4 structures in live cells. We also use the SG4 protein to positionally map G4s in situ and also on fixed chromatin. SG4 is a valuable, new tool for G4 detection and mapping in cells.
机构:
Univ Cambridge, Dept Chem, Cambridge CB2 1EW, England
Canc Res UK, Cambridge Res Inst, Li Ka Shing Ctr, Cambridge, EnglandUniv Cambridge, Dept Chem, Cambridge CB2 1EW, England
机构:
Univ Cambridge, Dept Chem, Cambridge CB2 1EW, England
Canc Res UK, Cambridge Res Inst, Li Ka Shing Ctr, Cambridge, EnglandUniv Cambridge, Dept Chem, Cambridge CB2 1EW, England