Kausik Chakraborty scite author profile

The GroEL/GroES chaperonin system mediates protein folding in the bacterial cytosol. Newly synthesized proteins reach GroEL via transfer from upstream chaperones such as DnaK/DnaJ (Hsp70). Here we employed single molecule and ensemble FRET to monitor the conformational transitions of a model substrate as it proceeds along this chaperone pathway. We find that DnaK/DnaJ stabilizes the protein in collapsed states that fold exceedingly slowly. Transfer to GroEL results in unfolding, with a fraction of molecules reaching locally highly expanded conformations. ATP-induced domain movements in GroEL cause transient further unfolding and rapid mobilization of protein segments with moderate hydrophobicity, allowing partial compaction on the GroEL surface. The more hydrophobic regions are released upon subsequent protein encapsulation in the central GroEL cavity by GroES, completing compaction and allowing rapid folding. Segmental chain release and compaction may be important in avoiding misfolding by proteins that fail to fold efficiently through spontaneous hydrophobic collapse.

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Chaperonin-Catalyzed Rescue of Kinetically Trapped States in Protein Folding

Chakraborty

Chatila

Sinha

et al. 2010

Cell

130

163

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GroEL and GroES form a chaperonin nano-cage for single protein molecules to fold in isolation. The folding properties that render a protein chaperonin dependent are not yet understood. Here, we address this question using a double mutant of the maltose-binding protein DM-MBP as a substrate. Upon spontaneous refolding, DM-MBP populates a kinetically trapped intermediate that is collapsed but structurally disordered. Introducing two long-range disulfide bonds into DM-MBP reduces the entropic folding barrier of this intermediate and strongly accelerates native state formation. Strikingly, steric confinement of the protein in the chaperonin cage mimics the kinetic effect of constraining disulfides on folding, in a manner mediated by negative charge clusters in the cage wall. These findings suggest that chaperonin dependence correlates with the tendency of proteins to populate entropically stabilized folding intermediates. The capacity to rescue proteins from such folding traps may explain the uniquely essential role of chaperonin cages within the cellular chaperone network.

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Chemical chaperones assist intracellular folding to buffer mutational variations

et al. 2012

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Hidden genetic variations harbor potential for the evolution of new traits. Molecular chaperones, that assist protein folding, may conceal genetic variations in protein coding regions. Here, we investigate if the chemical milieu of cells has the potential to alleviate intracellular protein folding; potentially implicating a role of osmolytes in concealing genetic variations. Using the model osmolyte TMAO, we uncover that it can buffer mutations that impose kinetic traps in the folding pathways of two model proteins. Using this information, we rationally designed TMAO-dependent mutants in vivo, starting from a TMAO-independent protein. Strikingly, we delineate different osmolytes to have a unique spectrum of buffered-mutations. Consequently, the chemical milieu of cells may alter the folding pathways of unique mutant variants in polymorphic populations and lead to unanticipated spectra of genetic buffering. KeywordsProtein folding; chaperone; chemical chaperone; Proteostasis; TMAO; genetic buffering; canalization Alterations in gene sequences are a major source of variation in protein structure and function leading to phenotypic variation 12 . Since native structures of proteins are only marginally stable, majority of non-conserved changes in the protein sequences lead to the formation of non-functional or metastable proteins 3,4 . Metastable proteins are functional under permissive conditions but are rendered inactive under special circumstances, which could be a major source of hidden genetic diversity, a phenomenon referred to as geneticcanalization 5 . Metastability, through canalization, may allow robust protein structures to adopt alternate conformations without losing in vivo activity; a significant step towards evolution of new protein function [6][7][8][9][10][11][12] . To establish this link we need to understand if protein folding modulators assist intracellular folding of metastable mutants.Since intracellular milieu is enriched with osmolytes that act as chemical chaperones, we asked if these could favor genetic canalization. Although there are preliminary reports of osmolyte dependent folding in vivo 13 ,14 ,15 , it is unknown if osmolytes affect canalization by assisting the folding of metastable proteins. Since osmolytes may also affect chaperone

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Essential role of the chaperonin folding compartment in vivo

Tang

Chang

Chakraborty

et al. 2008

EMBO J

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The GroEL/GroES chaperonin system of Escherichia coli forms a nano-cage allowing single protein molecules to fold in isolation. However, as the chaperonin can also mediate folding independently of substrate encapsulation, it remained unclear whether the folding cage is essential in vivo. To address this question, we replaced wild-type GroEL with mutants of GroEL having either a reduced cage volume or altered charge properties of the cage wall. A stepwise reduction in cage size resulted in a gradual loss of cell viability, although the mutants bound non-native protein efficiently. Strikingly, a mild reduction in cage size increased the yield and the apparent rate of green fluorescent protein folding, consistent with the view that an effect of steric confinement can accelerate folding. As shown in vitro, the observed acceleration of folding was dependent on protein encapsulation by GroES but independent of GroES cycling regulated by the GroEL ATPase. Altering the net-negative charge of the GroEL cage wall also strongly affected chaperonin function. Based on these findings, the GroEL/GroES compartment is essential for protein folding in vivo.

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