Cathepsin S: Difference between revisions

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Latest revision as of 13:42, 4 November 2018

Cathepsin S is a protein that in humans is encoded by the CTSS gene.^[1] Transcript variants utilizing alternative polyadenylation signals exist for this gene.^[1]

Cathepsin S is a member of the peptidase C1 family and is a lysosomal cysteine protease that may participate in the degradation of antigenic proteins to peptides for presentation to the MHC class II. Cathepsin S can function as an elastase over a broad pH range in alveolar macrophages.

Function

Cathepsin S is a lysosomal enzyme that belongs to the papain family of cysteine proteases. While a role in antigen presentation has long been recognized, it is now understood that cathepsin S has a role in itch and pain, or nociception . The nociceptive activity results from cathepsin S functioning as a signaling molecule via activation of protease-activated receptors 2 and 4 members of the G-protein coupled receptor family.^[2]

Cathepsin S is expressed by antigen presenting cells including macrophages, B-lymphocytes, dendritic cells and microglia. Cathepsin S is expressed by some epithelial cells. Its expression is markedly increased in human keratinocytes following stimulation with interferon-gamma and its expression is elevated in psoriatic keratinocytes due to stimulation by proinflammatory factors. In contrast, cortical thymic epithelial cells do not express cathepsin S.

While pH optima of many lysosomal proteases are acidic, cathepsin S is an exception. This enzyme remains catalytically active under the neutral pH and has pH optimum between the pH values 6.0 and 7.5. Many lysosomal proteases are trapped inside the lysosome due to a problem with their stability. In contrast, cathepsin S remains stable and has a physiological role outside the lysosome. Immune cells, including macrophages and microglia, secrete cathepsin S in response to inflammatory mediators including lipopolysaccharides, proinflammatory cytokines and neutrophils. In vitro, cathepsin S retains some enzyme activity in the presence of 3M urea. Cathepsin S is produced as a zymogen and is activated by processing.

The activity of cathepsin S is tightly regulated by its endogenous inhibitor, cystatin C, which also has a role in antigen presentation. Cystatin A and B have a lower activity compared to cystatin C.

The active cleavage sites -(-Val-Val-Arg-)- of cathepsin S are supposed to have at least two amino acids surrounding it from each side.

While lysosomal proteases terminally degrade proteins in lysosomes, cathepsin S has own distinctive physiological role.

Role in antigen presentation

This enzyme has a critical role in antigen presentation. Major histocompatibility complex class II molecules interact with small peptide fragments for presentation on the surface of antigen-presenting immune cells. Cathepsin S participates in the degradation of the invariant or Ii chain that prevents loading the antigen into the complex. This degradation occurs in the lysosome. Chronologically, action of cathepsin S follows two cleavages performed by aspartyl proteases. Cathepsin S cleaves the remaining fragment of Ii (IiP1) and leaves a small part of Ii known as CLIP which stays directly associated with the complex.

Proteolytic degradation of Ii is important since it facilitates dissociation of CLIP from MHC II and then, complex can load the selected antigen. After loading the antigen, MHC II molecule moves to the cell surface. Thus, we can speculate that overexpression of cathepsin S may lead to premature degradation of Ii, occasional loading of MHC II and an autoimmune attack. Contrary, inhibition of cathepsin S will lead to a delay in degradation of Ii and loading the antigen into MHC II as well as inappropriate presence of uncleaved Li-fragments in MHC II on the cell surface. It will impair and weaken the immune response. For instance, this kind of MHC II will not be very efficient to induce proliferation of T-cells.

In macrophages, cathepsin S can be replaced by cathepsin F.

Role in degradation of ECM

Secreted cathepsin S cleaves some extracellular matrix (ECM) proteins. Cathepsin S may be considered the most potent elastase known. The list of proposed cathepsin S substrates includes laminin, fibronectin elastin, osteocalcin and some collagens. It also cleaves chondroitin sulfate, heparan sulfate and proteoglycans of the basal membrane. Cathepsin S plays an active role in blood vessels permeability and angiogenesis due to its elastolytic and collagenolytic activities. For instance, cleavage of laminin-5 by cathepsin S leads to generation of proangiogenic peptides. The expression of cathepsin S can be triggered by proinflammatory factors secreted by tumor cells.

In tumorogenesis, cathepsin S promotes a tumor growth.

Role in cytokine regulation

Cathepsin S expression and activity has also been shown to be upregulated in the skin of psoriasis patients. Whether it has a definitive role in causing the pathology of psoriasis is as yet unknown, however in the same study it was shown to specially cleave and activate the psoriasis-associated proinflammatory cytokine IL-36γ^[3]

Nociception

Cathepsin S has a role in nociception, including itch and gastrointestinal pain. The mechanism by which cathepsin S leads to itch and pain is consistent with the capacity of this cysteine protease to activate protease-activated receptors 2 and 4.^[4]^[2]

Cathepsin S inhibitors

Synthetic inhibitors of cathepsin S participated in numerous preclinical studies for the immune disorders including rheumatoid arthritis. Currently, at least one of them participates in a clinical trial for psoriasis. LHVS (morpholinurea-leucine-homophenylalanine-vinylsulfone-phenyl) is the most extensively studied synthetic inhibitor of cathepsin S. IC50 of LHVS is about 5 nM. Inhibition of cathepsin S by LHVS has shown to be neuroprotective after traumatic brain injury.^[5] The list of commercial inhibitors also includes paecilopeptin (acetyl-Leu-Val-CHO) and some others.

Clinical significance

Cathepsin S has been shown to be a significant prognostic factor for patients with type IV astrocytomas (glioblastoma multiforme), and its inhibition has shown improvement in survival time by mean average 5 months. This is because the cysteine enzyme can no longer act together with other proteases to break up the brain extracellular matrix. So the spread of the tumor is halted. Scientists have just announced that this enzyme predicts death, as it has been shown to be associated with both heart disease and cancer.

References

↑ ^1.0 ^1.1 "Entrez Gene: CTSS cathepsin S".
↑ ^2.0 ^2.1 Reddy VB, Sun S, Azimi E, Elmariah SB, Dong X, Lerner EA (July 2015). "Redefining the concept of protease-activated receptors: cathepsin S evokes itch via activation of Mrgprs". Nature Communications. 6: 7864. doi:10.1038/ncomms8864. PMC 4520244. PMID 26216096.
↑ Ainscough JS, Macleod T, McGonagle D, Brakefield R, Baron JM, Alase A, Wittmann M, Stacey M (March 2017). "Cathepsin S is the major activator of the psoriasis-associated proinflammatory cytokine IL-36γ" (PDF). Proceedings of the National Academy of Sciences of the United States of America. 114 (13): E2748–E2757. doi:10.1073/pnas.1620954114. PMC 5380102. PMID 28289191.
↑ Elmariah SB, Reddy VB, Lerner EA (June 25, 2014). "Cathepsin S signals via PAR2 and generates a novel tethered ligand receptor agonist". PLoS One. 9 (6): e99702. doi:10.1371/journal.pone.0099702. PMC 4070910. PMID 24964046.
↑ Xu J, Wang H, Ding K, Lu X, Li T, Wang J, Wang C, Wang J (Oct 24, 2013). "Inhibition of cathepsin S produces neuroprotective effects after traumatic brain injury in mice". Mediators of Inflammation. 2013 (2013): 187873. doi:10.1155/2013/187873. PMC 3824312. PMID 24282339.

External links

The MEROPS online database for peptidases and their inhibitors: C01.034
BRENDA online database for enzymes: 3.4.22.27

[entrez-1] 1.0 ^1.1 "Entrez Gene: CTSS cathepsin S".

[ReferenceA-2] 2.0 ^2.1 Reddy VB, Sun S, Azimi E, Elmariah SB, Dong X, Lerner EA (July 2015). "Redefining the concept of protease-activated receptors: cathepsin S evokes itch via activation of Mrgprs". Nature Communications. 6: 7864. doi:10.1038/ncomms8864. PMC 4520244. PMID 26216096.

[3] Ainscough JS, Macleod T, McGonagle D, Brakefield R, Baron JM, Alase A, Wittmann M, Stacey M (March 2017). "Cathepsin S is the major activator of the psoriasis-associated proinflammatory cytokine IL-36γ" (PDF). Proceedings of the National Academy of Sciences of the United States of America. 114 (13): E2748–E2757. doi:10.1073/pnas.1620954114. PMC 5380102. PMID 28289191.

[4] Elmariah SB, Reddy VB, Lerner EA (June 25, 2014). "Cathepsin S signals via PAR2 and generates a novel tethered ligand receptor agonist". PLoS One. 9 (6): e99702. doi:10.1371/journal.pone.0099702. PMC 4070910. PMID 24964046.

[pmid24282339-5] Xu J, Wang H, Ding K, Lu X, Li T, Wang J, Wang C, Wang J (Oct 24, 2013). "Inhibition of cathepsin S produces neuroprotective effects after traumatic brain injury in mice". Mediators of Inflammation. 2013 (2013): 187873. doi:10.1155/2013/187873. PMC 3824312. PMID 24282339.

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@@ Line 1: / Line 1: @@
-<!-- The PBB_Controls template provides controls for Protein Box Bot, please see Template:PBB_Controls for details. -->
+{{Infobox_gene}}
-{{PBB_Controls
+'''Cathepsin S''' is a [[protein]] that in humans is encoded by the ''CTSS'' [[gene]].<ref name="entrez">{{cite web | title = Entrez Gene: CTSS cathepsin S| url = https://www.ncbi.nlm.nih.gov/sites/entrez?Db=gene&Cmd=ShowDetailView&TermToSearch=1520| accessdate = }}</ref> Transcript variants utilizing alternative polyadenylation signals exist for this gene.<ref name="entrez"/>
-| update_page = yes
-| require_manual_inspection = no
-| update_protein_box = yes
-| update_summary = yes
-| update_citations = yes
-}}
-<!-- The GNF_Protein_box is automatically maintained by Protein Box Bot.  See Template:PBB_Controls to Stop updates. -->
+Cathepsin S is a member of the peptidase C1 family and is a [[lysosome|lysosomal]] [[cysteine protease]] that may participate in the degradation of antigenic proteins to peptides for presentation to the [[MHC class II]]. Cathepsin S can function as an [[elastase]] over a broad pH range in [[pulmonary alveolus|alveolar]] [[macrophage]]s.
-{{GNF_Protein_box
- | image = PBB_Protein_CTSS_image.jpg
- | image_source = [[Protein_Data_Bank|PDB]] rendering based on 1glo.
- | PDB = {{PDB2|1glo}}, {{PDB2|1ms6}}, {{PDB2|1npz}}, {{PDB2|1nqc}}, {{PDB2|2c0y}}, {{PDB2|2f1g}}, {{PDB2|2fq9}}, {{PDB2|2fra}}, {{PDB2|2frq}}, {{PDB2|2ft2}}, {{PDB2|2fud}}, {{PDB2|2fye}}, {{PDB2|2g6d}}, {{PDB2|2g7y}}, {{PDB2|2h7j}}, {{PDB2|2hh5}}, {{PDB2|2hhn}}, {{PDB2|2hxz}}, {{PDB2|2op3}}
- | Name = Cathepsin S
- | HGNCid = 2545
- | Symbol = CTSS
- | AltSymbols =; MGC3886
- | OMIM = 116845
- | ECnumber =
- | Homologene = 20867
- | MGIid = 107341
- | GeneAtlas_image1 = PBB_GE_CTSS_202902_s_at_tn.png
- | GeneAtlas_image2 = PBB_GE_CTSS_202901_x_at_tn.png
- | Function = {{GNF_GO|id=GO:0004218 |text = cathepsin S activity}}
- | Component = {{GNF_GO|id=GO:0005576 |text = extracellular region}} {{GNF_GO|id=GO:0005764 |text = lysosome}} {{GNF_GO|id=GO:0016020 |text = membrane}}
- | Process = {{GNF_GO|id=GO:0006508 |text = proteolysis}} {{GNF_GO|id=GO:0006955 |text = immune response}}
- | Orthologs = {{GNF_Ortholog_box
-    | Hs_EntrezGene = 1520
-    | Hs_Ensembl = ENSG00000163131
-    | Hs_RefseqProtein = NP_004070
-    | Hs_RefseqmRNA = NM_004079
-    | Hs_GenLoc_db =
-    | Hs_GenLoc_chr = 1
-    | Hs_GenLoc_start = 148969296
-    | Hs_GenLoc_end = 149005057
-    | Hs_Uniprot = P25774
-    | Mm_EntrezGene = 13040
-    | Mm_Ensembl = ENSMUSG00000038642
-    | Mm_RefseqmRNA = NM_021281
-    | Mm_RefseqProtein = NP_067256
-    | Mm_GenLoc_db =
-    | Mm_GenLoc_chr = 3
-    | Mm_GenLoc_start = 95612190
-    | Mm_GenLoc_end = 95641804
-    | Mm_Uniprot = Q3U5K1
-  }}
-}}
-'''Cathepsin S''', also known as '''CTSS''', is a human [[gene]].<ref name="entrez">{{cite web | title = Entrez Gene: CTSS cathepsin S| url = http://www.ncbi.nlm.nih.gov/sites/entrez?Db=gene&Cmd=ShowDetailView&TermToSearch=1520| accessdate = }}</ref>
-<!-- The PBB_Summary template is automatically maintained by Protein Box Bot.  See Template:PBB_Controls to Stop updates. -->
+== Function ==
-{{PBB_Summary
+{{Unreferenced section|date=April 2012}}
-| section_title =
+Cathepsin S is a lysosomal enzyme that belongs to the [[papain]] family of [[cysteine protease]]s. While a role in antigen presentation has long been recognized, it is now understood that cathepsin S has a role in itch and pain, or nociception . The nociceptive activity results from cathepsin S functioning as a signaling molecule via activation of protease-activated receptors 2 and 4 members of the G-protein coupled receptor family.<ref name="ReferenceA">{{cite journal | vauthors = Reddy VB, Sun S, Azimi E, Elmariah SB, Dong X, Lerner EA | title = Redefining the concept of protease-activated receptors: cathepsin S evokes itch via activation of Mrgprs | journal = Nature Communications | volume = 6 | pages = 7864 | date = July 2015 | pmid = 26216096 | pmc = 4520244 | doi = 10.1038/ncomms8864 }}</ref>
-| summary_text = The protein encoded by this gene, a member of the peptidase C1 family, is a lysosomal cysteine proteinase that may participate in the degradation of antigenic proteins to peptides for presentation on MHC class II molecules. The encoded protein can function as an elastase over a broad pH range in alveolar macrophages. Transcript variants utilizing alternative polyadenylation signals exist for this gene.<ref name="entrez">{{cite web | title = Entrez Gene: CTSS cathepsin S| url = http://www.ncbi.nlm.nih.gov/sites/entrez?Db=gene&Cmd=ShowDetailView&TermToSearch=1520| accessdate = }}</ref>
-}}
-==See also==
+Cathepsin S is expressed by antigen presenting cells including [[macrophage]]s, [[B-lymphocyte]]s, [[dendritic cell]]s and [[microglia]]. Cathepsin S is expressed by some [[epithelial]] cells. Its expression is markedly increased in human keratinocytes following stimulation with interferon-gamma and its expression is elevated in [[psoriatic]] [[keratinocyte]]s due to stimulation by proinflammatory factors. In contrast, cortical thymic epithelial cells do not express cathepsin S.
+While pH optima of many lysosomal proteases are acidic, cathepsin S is an exception. This enzyme remains catalytically active under the neutral pH and has pH optimum between the pH values 6.0 and 7.5. Many lysosomal proteases are trapped inside the lysosome due to a problem with their stability. In contrast, cathepsin S remains stable and has a physiological role outside the lysosome. Immune cells, including macrophages and microglia, secrete cathepsin S in response to inflammatory mediators including lipopolysaccharides, proinflammatory cytokines and neutrophils. In vitro, cathepsin S retains some enzyme activity in the presence of 3M urea. Cathepsin S is produced as a zymogen and is activated by processing.
+The activity of cathepsin S is tightly regulated by its endogenous inhibitor, cystatin C, which also has a role in antigen presentation. [[Cystatin A]] and [[Cystatin B|B]] have a lower activity compared to cystatin C.
+The active cleavage sites -(-Val-Val-Arg-)- of cathepsin S are supposed to have at least two amino acids surrounding it from each side.
+While lysosomal proteases terminally degrade proteins in lysosomes, cathepsin S has own distinctive physiological role.
+== Role in antigen presentation ==
+This enzyme has a critical role in [[antigen presentation]]. Major histocompatibility complex class II molecules interact with small peptide fragments for presentation on the surface of antigen-presenting immune cells. Cathepsin S participates in the degradation of the invariant or Ii chain that prevents loading the antigen into the complex. This degradation occurs in the lysosome. Chronologically, action of cathepsin S follows two cleavages performed by [[aspartyl protease]]s. Cathepsin S cleaves the remaining fragment of Ii (IiP1) and leaves a small part of Ii known as CLIP which stays directly associated with the complex.
+Proteolytic degradation of Ii is important since it facilitates dissociation of CLIP from MHC II and then, complex can load the selected antigen. After loading the antigen, MHC II molecule moves to the cell surface.  Thus, we can speculate that overexpression of cathepsin S may lead to premature degradation of Ii, occasional loading of MHC II and an autoimmune attack. Contrary, inhibition of cathepsin S will lead to a delay in degradation of Ii and loading the antigen into MHC II as well as inappropriate presence of uncleaved Li-fragments in MHC II on the cell surface. It will impair and weaken the immune response. For instance, this kind of MHC II will not be very efficient to induce proliferation of T-cells.
+In macrophages, cathepsin S can be replaced by [[cathepsin F]].
+== Role in degradation of ECM ==
+Secreted cathepsin S cleaves some [[extracellular matrix]] (ECM) proteins. Cathepsin S may be considered the most potent elastase known. The list of proposed cathepsin S substrates includes [[laminin]], fibronectin elastin, [[osteocalcin]] and some [[collagen]]s. It also cleaves [[chondroitin sulfate]], [[heparan sulfate]] and [[proteoglycan]]s of the [[basal membrane]]. Cathepsin S plays an active role in blood vessels permeability and [[angiogenesis]] due to its elastolytic and collagenolytic activities. For instance, cleavage of laminin-5 by cathepsin S leads to generation of proangiogenic peptides. The expression of cathepsin S can be triggered by proinflammatory factors secreted by tumor cells.
+In [[tumorogenesis]], cathepsin S promotes a tumor growth.
+== Role in cytokine regulation ==
+Cathepsin S expression and activity has also been shown to be upregulated in the skin of [[psoriasis]] patients. Whether it has a definitive role in causing the pathology of psoriasis is as yet unknown, however in the same study it was shown to specially cleave and activate the psoriasis-associated proinflammatory cytokine [[IL36G|IL-36γ]]<ref>{{cite journal | vauthors = Ainscough JS, Macleod T, McGonagle D, Brakefield R, Baron JM, Alase A, Wittmann M, Stacey M | title = Cathepsin S is the major activator of the psoriasis-associated proinflammatory cytokine IL-36γ | journal = Proceedings of the National Academy of Sciences of the United States of America | volume = 114 | issue = 13 | pages = E2748-E2757 | date = March 2017 | pmid = 28289191 | pmc = 5380102 | doi = 10.1073/pnas.1620954114 | url = https://zenodo.org/record/889527/files/article.pdf }}</ref>
+== Nociception ==
+Cathepsin S has a role in [[nociception]], including itch and gastrointestinal pain. The mechanism by which cathepsin S leads to itch and pain is consistent with the capacity of this cysteine protease to activate protease-activated receptors 2 and 4.<ref>{{cite journal | vauthors = Elmariah SB, Reddy VB, Lerner EA | title = Cathepsin S signals via PAR2 and generates a novel tethered ligand receptor agonist | journal = PLoS One | volume = 9 | issue = 6 | pages = e99702 | date = June 25, 2014 | pmid = 24964046 | pmc = 4070910 | doi = 10.1371/journal.pone.0099702 }}</ref><ref name="ReferenceA"/>
+== Cathepsin S inhibitors ==
+{{Unreferenced section|date=April 2012}}
+Synthetic inhibitors of cathepsin S participated in numerous preclinical studies for the immune disorders including rheumatoid arthritis. Currently, at least one of them participates in a clinical trial for psoriasis.
+LHVS (morpholinurea-leucine-homophenylalanine-vinylsulfone-phenyl) is the most extensively studied synthetic inhibitor of cathepsin S. IC50 of LHVS is about 5 nM. Inhibition of cathepsin S by LHVS has shown to be neuroprotective after traumatic brain injury.<ref name="pmid24282339">{{cite journal | vauthors = Xu J, Wang H, Ding K, Lu X, Li T, Wang J, Wang C, Wang J | title = Inhibition of cathepsin S produces neuroprotective effects after traumatic brain injury in mice | journal = Mediators of Inflammation | volume = 2013 | issue = 2013 | pages = 187873 | date = Oct 24, 2013 | pmid = 24282339 | pmc = 3824312 | doi = 10.1155/2013/187873 }}</ref> The list of commercial inhibitors also includes paecilopeptin (acetyl-Leu-Val-CHO) and some others.
+== Clinical significance ==
+Cathepsin S has been shown to be a significant prognostic factor for patients with type IV [[astrocytomas]] (glioblastoma multiforme), and its inhibition has shown improvement in survival time by mean average 5 months. This is because the cysteine enzyme can no longer act together with other proteases to break up the brain extracellular matrix. So the spread of the tumor is halted. Scientists have just announced that this enzyme predicts death, as it has been shown to be associated with both heart disease and cancer.
+== See also ==
 *[[Cathepsin]]
-==References==
+== References ==
-{{reflist|2}}
+{{reflist|33em}}
-==Further reading==
-{{refbegin | 2}}
+== Further reading ==
-{{PBB_Further_reading
+{{refbegin|33em}}
-| citations =
+* {{cite journal | vauthors = Shi GP, Munger JS, Meara JP, Rich DH, Chapman HA | title = Molecular cloning and expression of human alveolar macrophage cathepsin S, an elastinolytic cysteine protease | journal = The Journal of Biological Chemistry | volume = 267 | issue = 11 | pages = 7258–62 | date = April 1992 | pmid = 1373132 | doi =  }}
-*{{cite journal  | author=Shi GP, Munger JS, Meara JP, ''et al.'' |title=Molecular cloning and expression of human alveolar macrophage cathepsin S, an elastinolytic cysteine protease. |journal=J. Biol. Chem. |volume=267 |issue= 11 |pages= 7258-62 |year= 1992 |pmid= 1373132 |doi=  }}
+* {{cite journal | vauthors = Wang J, Tsirka SE | title = Contribution of extracellular proteolysis and microglia to intracerebral hemorrhage | journal = Neurocrit Care | volume = 3 | issue = 1 | pages = 77–85 | pmid = 16159103 | doi =  10.1385/NCC:3:1:077 }}
-*{{cite journal  | author=Wiederanders B, Brömme D, Kirschke H, ''et al.'' |title=Phylogenetic conservation of cysteine proteinases. Cloning and expression of a cDNA coding for human cathepsin S. |journal=J. Biol. Chem. |volume=267 |issue= 19 |pages= 13708-13 |year= 1992 |pmid= 1377692 |doi=  }}
+* {{cite journal | vauthors = Wiederanders B, Brömme D, Kirschke H, von Figura K, Schmidt B, Peters C | title = Phylogenetic conservation of cysteine proteinases. Cloning and expression of a cDNA coding for human cathepsin S | journal = The Journal of Biological Chemistry | volume = 267 | issue = 19 | pages = 13708–13 | date = July 1992 | pmid = 1377692 | doi =  }}
-*{{cite journal  | author=Ritonja A, Colić A, Dolenc I, ''et al.'' |title=The complete amino acid sequence of bovine cathepsin S and a partial sequence of bovine cathepsin L. |journal=FEBS Lett. |volume=283 |issue= 2 |pages= 329-31 |year= 1991 |pmid= 2044774 |doi=  }}
+* {{cite journal | vauthors = Ritonja A, Colić A, Dolenc I, Ogrinc T, Podobnik M, Turk V | title = The complete amino acid sequence of bovine cathepsin S and a partial sequence of bovine cathepsin L | journal = FEBS Letters | volume = 283 | issue = 2 | pages = 329–31 | date = June 1991 | pmid = 2044774 | doi = 10.1016/0014-5793(91)80620-I }}
-*{{cite journal  | author=Munger JS, Haass C, Lemere CA, ''et al.'' |title=Lysosomal processing of amyloid precursor protein to A beta peptides: a distinct role for cathepsin S. |journal=Biochem. J. |volume=311 ( Pt 1) |issue=  |pages= 299-305 |year= 1995 |pmid= 7575468 |doi=  }}
+* {{cite journal | vauthors = Munger JS, Haass C, Lemere CA, Shi GP, Wong WS, Teplow DB, Selkoe DJ, Chapman HA | title = Lysosomal processing of amyloid precursor protein to A beta peptides: a distinct role for cathepsin S | journal = The Biochemical Journal | volume = 311 ( Pt 1) | issue = 1 | pages = 299–305 | date = October 1995 | pmid = 7575468 | pmc = 1136152 | doi =  }}
-*{{cite journal  | author=Lemere CA, Munger JS, Shi GP, ''et al.'' |title=The lysosomal cysteine protease, cathepsin S, is increased in Alzheimer's disease and Down syndrome brain. An immunocytochemical study. |journal=Am. J. Pathol. |volume=146 |issue= 4 |pages= 848-60 |year= 1995 |pmid= 7717452 |doi=  }}
+* {{cite journal | vauthors = Lemere CA, Munger JS, Shi GP, Natkin L, Haass C, Chapman HA, Selkoe DJ | title = The lysosomal cysteine protease, cathepsin S, is increased in Alzheimer's disease and Down syndrome brain. An immunocytochemical study | journal = The American Journal of Pathology | volume = 146 | issue = 4 | pages = 848–60 | date = April 1995 | pmid = 7717452 | pmc = 1869262 | doi =  }}
-*{{cite journal  | author=Hall A, Håkansson K, Mason RW, ''et al.'' |title=Structural basis for the biological specificity of cystatin C. Identification of leucine 9 in the N-terminal binding region as a selectivity-conferring residue in the inhibition of mammalian cysteine peptidases. |journal=J. Biol. Chem. |volume=270 |issue= 10 |pages= 5115-21 |year= 1995 |pmid= 7890620 |doi=  }}
+* {{cite journal | vauthors = Hall A, Håkansson K, Mason RW, Grubb A, Abrahamson M | title = Structural basis for the biological specificity of cystatin C. Identification of leucine 9 in the N-terminal binding region as a selectivity-conferring residue in the inhibition of mammalian cysteine peptidases | journal = The Journal of Biological Chemistry | volume = 270 | issue = 10 | pages = 5115–21 | date = March 1995 | pmid = 7890620 | doi = 10.1074/jbc.270.10.5115 }}
-*{{cite journal  | author=Balbín M, Hall A, Grubb A, ''et al.'' |title=Structural and functional characterization of two allelic variants of human cystatin D sharing a characteristic inhibition spectrum against mammalian cysteine proteinases. |journal=J. Biol. Chem. |volume=269 |issue= 37 |pages= 23156-62 |year= 1994 |pmid= 8083219 |doi=  }}
+* {{cite journal | vauthors = Balbín M, Hall A, Grubb A, Mason RW, López-Otín C, Abrahamson M | title = Structural and functional characterization of two allelic variants of human cystatin D sharing a characteristic inhibition spectrum against mammalian cysteine proteinases | journal = The Journal of Biological Chemistry | volume = 269 | issue = 37 | pages = 23156–62 | date = September 1994 | pmid = 8083219 | doi =  }}
-*{{cite journal  | author=Shi GP, Webb AC, Foster KE, ''et al.'' |title=Human cathepsin S: chromosomal localization, gene structure, and tissue distribution. |journal=J. Biol. Chem. |volume=269 |issue= 15 |pages= 11530-6 |year= 1994 |pmid= 8157683 |doi=  }}
+* {{cite journal | vauthors = Shi GP, Webb AC, Foster KE, Knoll JH, Lemere CA, Munger JS, Chapman HA | title = Human cathepsin S: chromosomal localization, gene structure, and tissue distribution | journal = The Journal of Biological Chemistry | volume = 269 | issue = 15 | pages = 11530–6 | date = April 1994 | pmid = 8157683 | doi =  }}
-*{{cite journal  | author=Turk B, Stoka V, Turk V, ''et al.'' |title=High-molecular-weight kininogen binds two molecules of cysteine proteinases with different rate constants. |journal=FEBS Lett. |volume=391 |issue= 1-2 |pages= 109-12 |year= 1996 |pmid= 8706894 |doi=  }}
+* {{cite journal | vauthors = Turk B, Stoka V, Turk V, Johansson G, Cazzulo JJ, Björk I | title = High-molecular-weight kininogen binds two molecules of cysteine proteinases with different rate constants | journal = FEBS Letters | volume = 391 | issue = 1-2 | pages = 109–12 | date = August 1996 | pmid = 8706894 | doi = 10.1016/0014-5793(96)00611-4 }}
-*{{cite journal  | author=Baumgrass R, Williamson MK, Price PA |title=Identification of peptide fragments generated by digestion of bovine and human osteocalcin with the lysosomal proteinases cathepsin B, D, L, H, and S. |journal=J. Bone Miner. Res. |volume=12 |issue= 3 |pages= 447-55 |year= 1997 |pmid= 9076588 |doi=  }}
+* {{cite journal | vauthors = Baumgrass R, Williamson MK, Price PA | title = Identification of peptide fragments generated by digestion of bovine and human osteocalcin with the lysosomal proteinases cathepsin B, D, L, H, and S | journal = Journal of Bone and Mineral Research | volume = 12 | issue = 3 | pages = 447–55 | date = March 1997 | pmid = 9076588 | doi = 10.1359/jbmr.1997.12.3.447 }}
-*{{cite journal  | author=Würl P, Taubert H, Meye A, ''et al.'' |title=Immunohistochemical and clinical evaluation of cathepsin expression in soft tissue sarcomas. |journal=Virchows Arch. |volume=430 |issue= 3 |pages= 221-5 |year= 1997 |pmid= 9099979 |doi=  }}
+* {{cite journal | vauthors = Würl P, Taubert H, Meye A, Dansranjavin T, Weber E, Günther D, Berger D, Schmidt H, Dralle H, Rath FW | title = Immunohistochemical and clinical evaluation of cathepsin expression in soft tissue sarcomas | journal = Virchows Archiv | volume = 430 | issue = 3 | pages = 221–5 | date = March 1997 | pmid = 9099979 | doi = 10.1007/BF01324805 }}
-*{{cite journal  | author=Gelb BD, Shi GP, Heller M, ''et al.'' |title=Structure and chromosomal assignment of the human cathepsin K gene. |journal=Genomics |volume=41 |issue= 2 |pages= 258-62 |year= 1997 |pmid= 9143502 |doi= 10.1006/geno.1997.4631 }}
+* {{cite journal | vauthors = Gelb BD, Shi GP, Heller M, Weremowicz S, Morton C, Desnick RJ, Chapman HA | title = Structure and chromosomal assignment of the human cathepsin K gene | journal = Genomics | volume = 41 | issue = 2 | pages = 258–62 | date = April 1997 | pmid = 9143502 | doi = 10.1006/geno.1997.4631 }}
-*{{cite journal  | author=Baldassare JJ, Henderson PA, Tarver A, Fisher GJ |title=Thrombin activation of human platelets dissociates a complex containing gelsolin and actin from phosphatidylinositide-specific phospholipase Cgamma1. |journal=Biochem. J. |volume=324 ( Pt 1) |issue=  |pages= 283-7 |year= 1997 |pmid= 9164868 |doi=  }}
+* {{cite journal | vauthors = Baldassare JJ, Henderson PA, Tarver A, Fisher GJ | title = Thrombin activation of human platelets dissociates a complex containing gelsolin and actin from phosphatidylinositide-specific phospholipase Cgamma1 | journal = The Biochemical Journal | volume = 324 ( Pt 1) | issue = 1 | pages = 283–7 | date = May 1997 | pmid = 9164868 | pmc = 1218428 | doi =  }}
-*{{cite journal  | author=Nissler K, Kreusch S, Rommerskirch W, ''et al.'' |title=Sorting of non-glycosylated human procathepsin S in mammalian cells. |journal=Biol. Chem. |volume=379 |issue= 2 |pages= 219-24 |year= 1998 |pmid= 9524075 |doi=  }}
+* {{cite journal | vauthors = Nissler K, Kreusch S, Rommerskirch W, Strubel W, Weber E, Wiederanders B | title = Sorting of non-glycosylated human procathepsin S in mammalian cells | journal = Biological Chemistry | volume = 379 | issue = 2 | pages = 219–24 | date = February 1998 | pmid = 9524075 | doi = 10.1515/bchm.1998.379.2.219 }}
-*{{cite journal  | author=Claus V, Jahraus A, Tjelle T, ''et al.'' |title=Lysosomal enzyme trafficking between phagosomes, endosomes, and lysosomes in J774 macrophages. Enrichment of cathepsin H in early endosomes. |journal=J. Biol. Chem. |volume=273 |issue= 16 |pages= 9842-51 |year= 1998 |pmid= 9545324 |doi=  }}
+* {{cite journal | vauthors = Claus V, Jahraus A, Tjelle T, Berg T, Kirschke H, Faulstich H, Griffiths G | title = Lysosomal enzyme trafficking between phagosomes, endosomes, and lysosomes in J774 macrophages. Enrichment of cathepsin H in early endosomes | journal = The Journal of Biological Chemistry | volume = 273 | issue = 16 | pages = 9842–51 | date = April 1998 | pmid = 9545324 | doi = 10.1074/jbc.273.16.9842 }}
-*{{cite journal  | author=Schick C, Pemberton PA, Shi GP, ''et al.'' |title=Cross-class inhibition of the cysteine proteinases cathepsins K, L, and S by the serpin squamous cell carcinoma antigen 1: a kinetic analysis. |journal=Biochemistry |volume=37 |issue= 15 |pages= 5258-66 |year= 1998 |pmid= 9548757 |doi= 10.1021/bi972521d }}
+* {{cite journal | vauthors = Schick C, Pemberton PA, Shi GP, Kamachi Y, Cataltepe S, Bartuski AJ, Gornstein ER, Brömme D, Chapman HA, Silverman GA | title = Cross-class inhibition of the cysteine proteinases cathepsins K, L, and S by the serpin squamous cell carcinoma antigen 1: a kinetic analysis | journal = Biochemistry | volume = 37 | issue = 15 | pages = 5258–66 | date = April 1998 | pmid = 9548757 | doi = 10.1021/bi972521d }}
-*{{cite journal  | author=Fengler A, Brandt W |title=Three-dimensional structures of the cysteine proteases cathepsins K and S deduced by knowledge-based modelling and active site characteristics. |journal=Protein Eng. |volume=11 |issue= 11 |pages= 1007-13 |year= 1999 |pmid= 9876921 |doi=  }}
+* {{cite journal | vauthors = Fengler A, Brandt W | title = Three-dimensional structures of the cysteine proteases cathepsins K and S deduced by knowledge-based modelling and active site characteristics | journal = Protein Engineering | volume = 11 | issue = 11 | pages = 1007–13 | date = November 1998 | pmid = 9876921 | doi = 10.1093/protein/11.11.1007 }}
-*{{cite journal  | author=Söderström M, Salminen H, Glumoff V, ''et al.'' |title=Cathepsin expression during skeletal development. |journal=Biochim. Biophys. Acta |volume=1446 |issue= 1-2 |pages= 35-46 |year= 1999 |pmid= 10395917 |doi=  }}
+* {{cite journal | vauthors = Söderström M, Salminen H, Glumoff V, Kirschke H, Aro H, Vuorio E | title = Cathepsin expression during skeletal development | journal = Biochimica et Biophysica Acta | volume = 1446 | issue = 1-2 | pages = 35–46 | date = July 1999 | pmid = 10395917 | doi = 10.1016/S0167-4781(99)00068-8 }}
-*{{cite journal  | author=Cao H, Hegele RA |title=Human cathepsin S gene (CTSS) promoter -25G/A polymorphism. |journal=J. Hum. Genet. |volume=45 |issue= 2 |pages= 94-5 |year= 2000 |pmid= 10721671 |doi=  }}
+* {{cite journal | vauthors = Cao H, Hegele RA | title = Human cathepsin S gene (CTSS) promoter -25G/A polymorphism | journal = Journal of Human Genetics | volume = 45 | issue = 2 | pages = 94–5 | year = 2000 | pmid = 10721671 | doi = 10.1007/s100380050019 }}
-*{{cite journal  | author=Luke C, Schick C, Tsu C, ''et al.'' |title=Simple modifications of the serpin reactive site loop convert SCCA2 into a cysteine proteinase inhibitor: a critical role for the P3' proline in facilitating RSL cleavage. |journal=Biochemistry |volume=39 |issue= 24 |pages= 7081-91 |year= 2000 |pmid= 10852705 |doi=  }}
+* {{cite journal | vauthors = Luke C, Schick C, Tsu C, Whisstock JC, Irving JA, Brömme D, Juliano L, Shi GP, Chapman HA, Silverman GA | title = Simple modifications of the serpin reactive site loop convert SCCA2 into a cysteine proteinase inhibitor: a critical role for the P3' proline in facilitating RSL cleavage | journal = Biochemistry | volume = 39 | issue = 24 | pages = 7081–91 | date = June 2000 | pmid = 10852705 | doi = 10.1021/bi000050g }}
-}}
 {{refend}}
-{{protein-stub}}
+== External links ==
+* The [[MEROPS]] online database for peptidases and their inhibitors: [http://merops.sanger.ac.uk/cgi-bin/merops.cgi?id=C01.034 C01.034]
+* {{BRENDA|3.4.22.27}}
+{{PDB Gallery|geneid=1520}}
+{{Cysteine proteases}}
+{{Enzymes}}
+{{Portal bar|Molecular and Cellular Biology|border=no}}
+[[Category:Peptidase]]
+[[Category:EC 3.4.22]]

v t e Proteases: cysteine proteases (EC 3.4.22)
Caspase	Caspase 1 Caspase 2 Caspase 3 Caspase 4 Caspase 5 Caspase 6 Caspase 7 Caspase 8 Caspase 9 Caspase 10 Caspase 12 Caspase 13 Caspase 14
Fruit-derived	Papain Ficain Bromelain Actinidain
Calpain	CAPN1 CAPN2 CAPN3 CAPN5 CAPN6 CAPN7 CAPN8 CAPN9 CAPN10 CAPN11 CAPN12 CAPN13 CAPN14 CAPNS1 CAPNS2
Cathepsin	B C F H K L1/L2 O S W Z
Other	Clostripain Cancer procoagulant Separase Autophagin Cruzipain

v t e Enzymes
Activity	Active site Binding site Catalytic triad Oxyanion hole Enzyme promiscuity Catalytically perfect enzyme Coenzyme Cofactor Enzyme catalysis
Regulation	Allosteric regulation Cooperativity Enzyme inhibitor Enzyme activator
Classification	EC number Enzyme superfamily Enzyme family List of enzymes
Kinetics	Enzyme kinetics Eadie–Hofstee diagram Hanes–Woolf plot Lineweaver–Burk plot Michaelis–Menten kinetics
Types	EC1 Oxidoreductases (list) EC2 Transferases (list) EC3 Hydrolases (list) EC4 Lyases (list) EC5 Isomerases (list) EC6 Ligases (list)