Gene editing of SAMHD1 in macrophage-like cells reveals complex relationships between SAMHD1 phospho-regulation, HIV-1restriction,andcellulardNTPlevelsHIV-1 restriction, and cellular dNTP levels
Sterile a motif and HD domain-containing protein 1 (SAMHD1) is a dNTP triphosphate triphosphohydrolase (dNTPase) and a potent restriction factor for immuno deficiency virus 1 (HIV-1), active in myeloid and resting CD4(+) T cells. The anti-viral activity of SAMHD1 is regulated by dephosphorylation of the residue T592. However, the impact of T592 phosphorylation on dNTPase activity is still under debate. Whether additional cellular functions of SAMHD1 impact anti-viral restriction is not completely understood. We report BLaER1 cells as a novel human macrophage HIV-1 infection model combined with CRISPR/Cas9 knock-in (KI) introducing specific mutations into the SAMHD1 locus to study mutations in a physiological context. Transdifferentiated BLaER1 cells harbor active dephosphorylated SAMHD1 that blocks HIV-1 reporter virus infection. As expected, homozygous T592E mutation, but not T592A, relieved a block to HIV-1 reverse transcription. Co-delivery of VLP-Vpx to SAMHD1 T592E KI mutant cells did not further enhance HIV-1 infection indicating the absence of additional SAMHD1-mediated anti-viral activity independent of T592 dephosphorylation. T592E KI cells retained dNTP levels similar to WT cells indicating uncoupling of anti-viral and dNTPase activity of SAMHD1. The integrity of the catalytic site in SAMHD1 was critical for anti-viral activity, yet a poor correlation between HIV-1 restriction and global cellular dNTP levels was observed in cells harboring catalytic core mutations. Together, we emphasize the complexity of the relationship between HIV-1 restriction, SAMHD1 enzymatic function, and T592 phospho-regulation and provide novel tools for investigation in an endogenous and physiological context. IMPORTANCE We introduce BLaER1 cells as an alternative myeloid cell model in combination with CRISPR/Cas9-mediated gene editing to study the influence of sterile a motif and HD domain-containing protein 1 (SAMHD1) T592 phosphorylation on anti-viral restriction and the control of cellular dNTP levels in an endogenous, physiologically relevant context. A proper understanding of the mechanism of the anti-viral function of SAMHD1 will provide attractive strategies aiming at selectively manipulating SAMHD1 without affecting other cellular functions. Even more, our toolkit may inspire further genetic analysis and investigation of restriction factors inhibiting retroviruses and their cellular function and regulation, leading to a deeper understanding of intrinsic anti-viral immunity.
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Francis Crick Inst, Mill Hill Lab, London, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
Arnold, Laurence H.
Groom, Harriet C. T.
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Francis Crick Inst, Mill Hill Lab, London, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
Groom, Harriet C. T.
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Kunzelmann, Simone
Schwefel, David
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Francis Crick Inst, Mill Hill Lab, London, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
Schwefel, David
Caswell, Sarah J.
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Francis Crick Inst, Mill Hill Lab, London, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
Caswell, Sarah J.
Ordonez, Paula
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Francis Crick Inst, Mill Hill Lab, London, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
Ordonez, Paula
Mann, Melanie C.
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Francis Crick Inst, Mill Hill Lab, London, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
Mann, Melanie C.
Rueschenbaum, Sabrina
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Francis Crick Inst, Mill Hill Lab, London, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
Rueschenbaum, Sabrina
Goldstone, David C.
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Francis Crick Inst, Mill Hill Lab, London, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
Goldstone, David C.
Pennell, Simon
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Francis Crick Inst, Mill Hill Lab, London, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
Pennell, Simon
Howell, Steven A.
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Francis Crick Inst, Mill Hill Lab, London, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
Howell, Steven A.
Stoye, Jonathan P.
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Francis Crick Inst, Mill Hill Lab, London, England
Univ London Imperial Coll Sci Technol & Med, Fac Med, London, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
Stoye, Jonathan P.
Webb, Michelle
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Univ Manchester, Fac Med & Human Sci, Inst Human Dev, Ctr Genom Med, Manchester, Lancs, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
Webb, Michelle
Taylor, Ian A.
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Francis Crick Inst, Mill Hill Lab, London, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
Taylor, Ian A.
Bishop, Kate N.
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Francis Crick Inst, Mill Hill Lab, London, EnglandFrancis Crick Inst, Mill Hill Lab, London, England
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Francis Crick Inst, Retroviral Replicat Lab, London, England
LabGenius, London, EnglandFrancis Crick Inst, Retroviral Replicat Lab, London, England
Tsai, Ming-Han C.
Caswell, Sarah J.
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Francis Crick Inst, Macromol Struct Lab, London, England
AstraZeneca, Granta Pk, Cambridge, EnglandFrancis Crick Inst, Retroviral Replicat Lab, London, England
Caswell, Sarah J.
Morris, Elizabeth R.
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Francis Crick Inst, Macromol Struct Lab, London, England
Univ Durham, Dept Biosci, Durham, EnglandFrancis Crick Inst, Retroviral Replicat Lab, London, England
Morris, Elizabeth R.
Mann, Melanie C.
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Francis Crick Inst, Retroviral Replicat Lab, London, England
Sartorius, Ulm, GermanyFrancis Crick Inst, Retroviral Replicat Lab, London, England
Mann, Melanie C.
Pennell, Simon
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Francis Crick Inst, Struct Biol DNA Damage Signalling Lab, London, England
MRC London Inst Med Sci, London, EnglandFrancis Crick Inst, Retroviral Replicat Lab, London, England
Pennell, Simon
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Kelly, Geoff
Groom, Harriet C. T.
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Francis Crick Inst, Retroviral Replicat Lab, London, England
Univ Cambridge, Dept Med, Cambridge, EnglandFrancis Crick Inst, Retroviral Replicat Lab, London, England
Groom, Harriet C. T.
Taylor, Ian A.
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Francis Crick Inst, Macromol Struct Lab, London, EnglandFrancis Crick Inst, Retroviral Replicat Lab, London, England
Taylor, Ian A.
Bishop, Kate N.
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Francis Crick Inst, Retroviral Replicat Lab, London, EnglandFrancis Crick Inst, Retroviral Replicat Lab, London, England