Biology:ClpX
Generic protein structure example |
ATP-dependent Clp protease ATP-binding subunit clpX-like, mitochondrial is an enzyme that in humans is encoded by the CLPX gene. This protein is a member of the family of AAA Proteins (AAA+ ATPase) and is to form the protein complex of Clp protease (Endopeptidase Clp).
Structure
Tertiary
The human enzyme ClpX is drawn from the protein complex structure of Clp protease. These hexameric HSP100/Clp proteins produce ring like structures resembling chaperonins.[1]
The Clp proteases have a two-component structure which includes two different proteolytic cores and multiple chaperone rings. As a result, there are several possible combinations of Clp protease complexes. The ClpP protease core can partner with different chaperones, namely ClpA, ClpC, ClpE, and ClpX, to form active chaperone-protease complexes. On the other hand, ClpQ interacts exclusively with the ClpY chaperone to form the ClpYQ protease (also called HslUV) . The Clp-type ATPases can be classified into two distinct groups: class I with two consecutive AAA modules per protomer(ClpA, ClpC, and ClpE) and class II with only one AAA module per protomer.[2]
ClpA and ClpX of E. coli are protein unfoldases that require ATP to function. They individually associate with the ClpP protease to facilitate targeted protein degradation.[3] These variants have inflicted variants interspecific with ClpP.
Quaternary
The complex assembly of the regulatory subunits of ATP-dependent Clp proteases is induced in the critical role in cellular thermotolerance. There are numerous proteases that are thought to have a bacterial origin. Studies on the protein of E. coli are the main source of information about the human ClpX protein. In E. coli, the ClpX protein monomer has an N-terminal domain and a AAA+ module made up of two AAA+ domains, one larger than the other.[4] Since the prevalence of E.coli is at such a high factor in most people around the world, the constitutive aspect of ClpX showed multiple signs in research of the protease.
Clp protease is made up of ATPase-active chaperone rings and a proteolytic core, two functional units with distinct functions that play a role in cellular thermotolerance.[5][6] The ClpXP chaperone-protease is present in almost every type of bacteria, commonly found together with the widely distributed Lon and FtsH proteases. Hence, ClpXP is the most prevalent among the Clp.[7]
The HslV rings engage with an unrelated chaperone ATPase called HslU, which also has 6-fold ring symmetry. This is similar to the ClpX chaperone, which it potentially evolved from, and almost all AAA+ ATPase proteins that emerged from a surge of gene duplications prior to the last common ancestor of all life. This allows the assumption that most mammals from the common ancestors between humans and mice were shown to have this relating enzyme. As shown on the infobox gene similarity between a mouse and a human, we can distinctly see its similarities and differences in the Clp protease.
Function
Bacteria use the ATP-dependent ClpX protease for a variety of purposes, including protein quality control, stress tolerance, the production of virulence factors, and binding to protein degradation tags in E.coli. The ATPase component is in charge of substrate recognition, unfolding, and transport into the proteolytic component. The proteolytic component has several serine- or threonine-type active sites that allow for protein hydrolysis. [8] Accordingly, it seems that depending on the physiological circumstances, clpX can either be produced alone or in conjunction with clpP in cells.[9] ClpX and ClpP are two proteins that work together in the ClpXP complex, which is a major protein degradation system in bacteria. ClpX is an ATPase that provides the energy for unfolding and translocating target proteins into the ClpP protease for degradation. ClpP is the protease that cleaves the unfolded target proteins.
The function of the ClpX has several complexity factors that can be seen in the proteasome evolution figure. This shows the evolution of proteasomes that has occurred in a stepwise manner, with increasing complexity over time. The first step was the development of the HslV ring protease, followed by the 20S proteasome, and finally, the 26S proteasome. Grey bars on the evolutionary tree represent the two significant transitions in proteasome structure that are crucial for polarizing the tree. Additionally, four other evolutionary transitions are marked by blue bars that also align with the tree's polarization. The HslV ring protease has 6-fold symmetry, with a 2-tiered ring consisting of 12 identical subunits. It is believed to have arisen from a monomeric NTN hydrolase, possibly just before the divergence of Hadobacteria.[10] The regulation of ClpX and ClpP expression is complex and involves various factors, including transcriptional regulators, environmental signals, and post-transcriptional modifications. Understanding how the expression of these proteins is regulated can provide insights into the mechanisms by which bacteria respond to stress and maintain cellular homeostasis.
Clinical significance
The mitochondrial system responsible for maintaining protein quality, especially clpx, plays a crucial role in influencing fertility, survival, and neural aging. [11] Studies have indicated that improper regulation of the protein quality control system within the mitochondria, which includes the CLPXP complex, can significantly impact cellular health and function. For instance, when researchers deleted the CLPP subunit in mice, they observed a decline in fertility and a rise in early embryonic mortality. These findings suggest that the clpx complex plays a crucial role in maintaining appropriate mitochondrial function during gamete production and embryonic development.
The ClpXP protease is a significant player in mitochondrial protein quality control in mammals. When ClpXP function is compromised, it can result in the accumulation of damaged proteins and mitochondrial malfunctions. These issues are believed to be potential causes of neurodegenerative diseases and aging. Having such a variety of Clp complexes, the insight of the ClpX assembly is crucial to identify any detrimental damages in humans for long term issues or term. Having a common ancestor with mice allows for future studies to be developed in understanding this enzyme.
Through extensive research of E.coli with correlation to ClpXp, research on Mycobacterium tuberculosis took place. The data revealed that ClpX participates in DNA replication and identify the first activator of ClpXp in mycobacteria as well.[12] This knowledge correlates with research of when ClpX is inhibited, the bacterium became more susceptible to antibiotics. This suggests that targeting ClpX could be a strategy for overcoming antibiotic resistance in bacterial infections in this research. However, the research is ongoing and more definitive results are needed to take place.
References
- ↑ "Mcx1p, a ClpX homologue in mitochondria of Saccharomyces cerevisiae". FEBS Letters 438 (3): 250–254. November 1998. doi:10.1016/s0014-5793(98)01310-6. PMID 9827555.
- ↑ "Functional domains of the ClpA and ClpX molecular chaperones identified by limited proteolysis and deletion analysis". The Journal of Biological Chemistry 276 (31): 29420–29429. August 2001. doi:10.1074/jbc.M103489200. PMID 11346657.
- ↑ "ClpX, an alternative subunit for the ATP-dependent Clp protease of Escherichia coli. Sequence and in vivo activities". The Journal of Biological Chemistry 268 (30): 22618–22626. October 1993. doi:10.1016/S0021-9258(18)41573-6. PMID 8226770.
- ↑ "Plant mitochondria contain proteolytic and regulatory subunits of the ATP-dependent Clp protease". Plant Molecular Biology 45 (4): 461–468. March 2001. doi:10.1023/A:1010677220323. PMID 11352464.
- ↑ "Principles of general and regulatory proteolysis by AAA+ proteases in Escherichia coli". Research in Microbiology 160 (9): 629–36. November 2009. doi:10.1016/j.resmic.2009.08.018. PMID 19781640.
- ↑ "Clp chaperone-proteases: structure and function". Research in Microbiology 160 (9): 618–28. November 2009. doi:10.1016/j.resmic.2009.08.006. PMID 19732826.
- ↑ "Clp chaperone-proteases: structure and function". Research in Microbiology. Special issue on proteolysis in prokaryotes: protein quality control and regulatory principles 160 (9): 618–628. November 2009. doi:10.1016/j.resmic.2009.08.006. PMID 19732826.
- ↑ "Clp chaperone-proteases: structure and function". Research in Microbiology. Special issue on proteolysis in prokaryotes: protein quality control and regulatory principles 160 (9): 618–628. November 2009. doi:10.1016/j.resmic.2009.08.006. PMID 19732826.
- ↑ "clpX encoding an alternative ATP-binding subunit of protease Ti (Clp) can be expressed independently from clpP in Escherichia coli". Biochemical and Biophysical Research Communications 203 (2): 798–804. September 1994. doi:10.1006/bbrc.1994.2253. PMID 8093059.
- ↑ "File:Rooting-the-tree-of-life-by-transition-analyses-1745-6150-1-19-5.jpg - Wikipedia" (in en). https://commons.wikimedia.org/wiki/File:Rooting-the-tree-of-life-by-transition-analyses-1745-6150-1-19-5.jpg.
- ↑ "Quality control of mitochondria: protection against neurodegeneration and ageing". The EMBO Journal 27 (2): 306–314. January 2008. doi:10.1038/sj.emboj.7601972. PMID 18216873.
- ↑ "ClpX Is Essential and Activated by Single-Strand DNA Binding Protein in Mycobacteria". Journal of Bacteriology 203 (4). January 2021. doi:10.1128/JB.00608-20. PMID 33229461.
Original source: https://en.wikipedia.org/wiki/ClpX.
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