Nadine Renner scite author profile

Trim-Away is a recently developed technology that exploits off-the-shelf antibodies and the E3 RING ligase and cytosolic antibody receptor TRIM21 to carry out rapid protein depletion. How TRIM21 is catalytically activated upon target engagement, either during its normal immune function or when re-purposed for targeted protein degradation, is unknown. Here we show that a mechanism of target-induced clustering triggers intermolecular dimerisation of the RING domain, to switch on the ubiquitination activity of TRIM21 and induce virus neutralisation or drive Trim-Away. We harness this mechanism for selective degradation of disease-causing huntingtin protein containing long polyQ tracts, and expand the Trim-Away toolbox with highly active TRIM21-nanobody chimeras that can also be controlled optogenetically. This work provides a mechanism for cellular activation of TRIM RING ligases and has implications for targeted protein degradation technologies.

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RING domains act as both substrate and enzyme in a catalytic arrangement to drive self-anchored ubiquitination

Kiss

Clift

Renner

et al. 2021

Nat Commun

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Attachment of ubiquitin (Ub) to proteins is one of the most abundant and versatile of all posttranslational modifications and affects outcomes in essentially all physiological processes. RING E3 ligases target E2 Ub-conjugating enzymes to the substrate, resulting in its ubiquitination. However, the mechanism by which a ubiquitin chain is formed on the substrate remains elusive. Here we demonstrate how substrate binding can induce a specific RING topology that enables self-ubiquitination. By analyzing a catalytically trapped structure showing the initiation of TRIM21 RING-anchored ubiquitin chain elongation, and in combination with a kinetic study, we illuminate the chemical mechanism of ubiquitin conjugation. Moreover, biochemical and cellular experiments show that the topology found in the structure can be induced by substrate binding. Our results provide insights into ubiquitin chain formation on a structural, biochemical and cellular level with broad implications for targeted protein degradation.

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A stable immature lattice packages IP ₆ for HIV capsid maturation

et al. 2021

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HIV virion assembly begins with the construction of an immature lattice consisting of Gag hexamers. Upon virion release, protease-mediated Gag cleavage leads to a maturation event in which the immature lattice disassembles and the mature capsid assembles. The cellular metabolite inositiol hexakisphosphate (IP6) and maturation inhibitors (MIs) both bind and stabilize immature Gag hexamers, but whereas IP6 promotes virus maturation, MIs inhibit it. Here we show that HIV is evolutionarily constrained to maintain an immature lattice stability that ensures IP6 packaging without preventing maturation. Replication-deficient mutant viruses with reduced IP6 recruitment display increased infectivity upon treatment with the MI PF46396 (PF96) or the acquisition of second-site compensatory mutations. Both PF96 and second-site mutations stabilise the immature lattice and restore IP6 incorporation, suggesting that immature lattice stability and IP6 binding are interdependent. This IP6 dependence suggests that modifying MIs to compete with IP6 for Gag hexamer binding could substantially improve MI antiviral potency.

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A lysine ring in HIV capsid pores coordinates IP6 to drive mature capsid assembly

et al. 2021

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The HIV capsid self-assembles a protective conical shell that simultaneously prevents host sensing whilst permitting the import of nucleotides to drive DNA synthesis. This is accomplished through the construction of dynamic, highly charged pores at the centre of each capsid multimer. The clustering of charges required for dNTP import is strongly destabilising and it is proposed that HIV uses the metabolite IP6 to coordinate the pore during assembly. Here we have investigated the role of inositol phosphates in coordinating a ring of positively charged lysine residues (K25) that forms at the base of the capsid pore. We show that whilst IP5, which can functionally replace IP6, engages an arginine ring (R18) at the top of the pore, the lysine ring simultaneously binds a second IP5 molecule. Dose dependent removal of K25 from the pore severely inhibits HIV infection and concomitantly prevents DNA synthesis. Cryo-tomography reveals that K25A virions have a severe assembly defect that inhibits the formation of mature capsid cones. Monitoring both the kinetics and morphology of capsids assembled in vitro reveals that while mutation K25A can still form tubes, the ability of IP6 to drive assembly of capsid cones has been lost. Finally, in single molecule TIRF microscopy experiments, capsid lattices in permeabilised K25 mutant virions are rapidly lost and cannot be stabilised by IP6. These results suggest that the coordination of IP6 by a second charged ring in mature hexamers drives the assembly of conical capsids capable of reverse transcription and infection.

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HIV-1 is dependent on its immature lattice to recruit IP6 for mature capsid assembly

Renner

Kleinpeter

Mallery

et al. 2023

Nat Struct Mol Biol

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IP6‐stabilised HIV capsids evade cGAS/STING‐mediated host immune sensing

et al. 2023

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HIV‐1 uses inositol hexakisphosphate (IP6) to build a metastable capsid capable of delivering its genome into the host nucleus. Here, we show that viruses that are unable to package IP6 lack capsid protection and are detected by innate immunity, resulting in the activation of an antiviral state that inhibits infection. Disrupting IP6 enrichment results in defective capsids that trigger cytokine and chemokine responses during infection of both primary macrophages and T‐cell lines. Restoring IP6 enrichment with a single mutation rescues the ability of HIV‐1 to infect cells without being detected. Using a combination of capsid mutants and CRISPR‐derived knockout cell lines for RNA and DNA sensors, we show that immune sensing is dependent upon the cGAS–STING axis and independent of capsid detection. Sensing requires the synthesis of viral DNA and is prevented by reverse transcriptase inhibitors or reverse transcriptase active‐site mutation. These results demonstrate that IP6 is required to build capsids that can successfully transit the cell and avoid host innate immune sensing.

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Pharmacologic hyperstabilisation of the HIV-1 capsid lattice induces capsid failure

Faysal

Renner

Márquez

et al. 2022

Preprint

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The HIV-1 capsid has emerged as a tractable target for antiretroviral therapy. Lenacapavir, developed by Gilead Sciences, is the first capsid-targeting drug approved for medical use. Here we investigate the effect of Lenacapavir on HIV capsid stability and uncoating. We employ a single particle approach that simultaneously measures capsid content release and lattice persistence. We demonstrate that Lenacapavir's potent antiviral activity is predominantly due to lethal hyperstabilisation of the capsid lattice and resultant loss of compartmentalisation. This study highlights that disrupting capsid metastability is a powerful strategy for the development of novel antivirals.

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Substrate-induced clustering activates Trim-Away of pathogens and proteins

Zeng

Santos

Mukadam

et al. 2020

Preprint

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SUMMARYTrim-Away is a powerful new technology that exploits off-the-shelf antibodies and the E3 RING ligase and cytosolic antibody receptor TRIM21 to carry out rapid protein depletion. How TRIM21 is catalytically-activated upon substrate engagement during either its normal immune function or when re-purposed for targeted protein degradation is unknown. Here we show that a mechanism of substrate-induced clustering triggers intermolecular dimerization of the RING domain to switch on the ubiquitination activity of TRIM21 and induce an antiviral response or drive Trim-Away. We harness this mechanism to expand the Trim-Away toolbox with highly-active TRIM21-nanobody chimeras that can also be controlled optogenetically. This work provides a mechanism for cellular activation of TRIM RING ligases and has important implications for targeted protein degradation technologies.

show abstract

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Nadine Renner

Target-induced clustering activates Trim-Away of pathogens and proteins

RING domains act as both substrate and enzyme in a catalytic arrangement to drive self-anchored ubiquitination

A stable immature lattice packages IP ₆ for HIV capsid maturation

A lysine ring in HIV capsid pores coordinates IP6 to drive mature capsid assembly

HIV-1 is dependent on its immature lattice to recruit IP6 for mature capsid assembly

IP6‐stabilised HIV capsids evade cGAS/STING‐mediated host immune sensing

Pharmacologic hyperstabilisation of the HIV-1 capsid lattice induces capsid failure

Substrate-induced clustering activates Trim-Away of pathogens and proteins

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Nadine Renner

Target-induced clustering activates Trim-Away of pathogens and proteins

RING domains act as both substrate and enzyme in a catalytic arrangement to drive self-anchored ubiquitination

A stable immature lattice packages IP 6 for HIV capsid maturation

A lysine ring in HIV capsid pores coordinates IP6 to drive mature capsid assembly

HIV-1 is dependent on its immature lattice to recruit IP6 for mature capsid assembly

IP6‐stabilised HIV capsids evade cGAS/STING‐mediated host immune sensing

Pharmacologic hyperstabilisation of the HIV-1 capsid lattice induces capsid failure

Substrate-induced clustering activates Trim-Away of pathogens and proteins

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Product

Resources

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A stable immature lattice packages IP ₆ for HIV capsid maturation