Abstract
The human pathogen Mycobacterium tuberculosis (Mtb) harbors a well-orchestrated Clp (caseinolytic protease) proteolytic machinery consisting of two oligomeric segments, a barrel-shaped heterotetradecameric protease core comprising the ClpP1 and ClpP2 subunits, and hexameric ring-like ATP-dependent unfoldases composed of ClpX or ClpC1. The roles of the ClpP1P2 protease subunits are well-established in Mtb, but the potential roles of the associated unfoldases, such as ClpC1, remain elusive. Using a CRISPR interference-mediated gene silencing approach, here we demonstrate that clpC1 is indispensable for the extracellular growth of Mtb and for its survival in macrophages. The results from isobaric tags for relative and absolute quantitation-based quantitative proteomic experiments with clpC1- and clpP2-depleted Mtb cells suggested that the ClpC1P1P2 complex critically maintains the homeostasis of various growth-essential proteins in Mtb, several of which contain intrinsically disordered regions at their termini. We show that the Clp machinery regulates dosage-sensitive proteins such as the small heat shock protein Hsp20, which exists in a dodecameric conformation. Further, we observed that Hsp20 is poorly expressed in WT Mtb and that its expression is greatly induced upon depletion of clpC1 or clpP2 Remarkably, high Hsp20 protein levels were detected in the clpC1(-) or clpP2(-) knockdown strains but not in the parental bacteria, despite significant induction of hsp20 transcripts. In summary, the cellular levels of oligomeric proteins such as Hsp20 are maintained post-translationally through their recognition, disassembly, and degradation by ClpC1, which requires disordered ends in its protein substrates.
Highlights
Stringent control of protein expression in a pathogen during regular growth condition, as well as in response to extracellular stimuli during infection, is an important determinant of its virulence (1)
We show that the small heat shock protein Hsp[20], which is highly accumulated in clpC1(2) and clpP2(2) strains of Mycobacterium tuberculosis (Mtb), is a dosage-sensitive protein, and its expression is maintained in Mtb exclusively by ClpC1P1P2 proteolytic machinery by recognition of its C-terminal region, which is disordered
ClpC1 unfoldase is essential for Mtb proliferation
Summary
Stringent control of protein expression in a pathogen during regular growth condition, as well as in response to extracellular stimuli during infection, is an important determinant of its virulence (1). The ATPases perform the maintenance function (5), whereas proteases act as final executioners in the life cycle of proteins (6) Known cases of such multicompartmentalized systems such as Clp (caseinolytic protease), Lon protease, or 20S proteasome reveal that the executory nature of proteases is managed by their fundamental architecture comprising of multisubunit chambered structure with a central pore, whereas associated ATPases such as ClpX, ClpA, ClpC1, or 19S proteasome, which are commonly known as unfoldases, recognize, unfold, and translocate the prospective substrate proteins into the proteolytic chamber (7). We show that the small heat shock protein Hsp[20], which is highly accumulated in clpC1(2) and clpP2(2) strains of Mtb, is a dosage-sensitive protein, and its expression is maintained in Mtb exclusively by ClpC1P1P2 proteolytic machinery by recognition of its C-terminal region, which is disordered
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