Acrosin

Acrosin is a digestive enzyme that acts as a protease. In humans, acrosin is encoded by the ACR gene.^[1]^[2] Acrosin is released from the acrosome of spermatozoa as a consequence of the acrosome reaction. It aids in the penetration of the Zona Pellucida.

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Enzyme Mechanism

Acrosin is a typical serine proteinase with trypsin-like specificity.^[3]

The reaction proceeds according to the usual serine protease mechanism. First, His-57 deprotonates Ser-195, allowing it to serve as a nucleophile. Deprotonated Ser-195 then reacts with the carbonyl carbon of a peptide, forming a tetrahedral intermediate. The tetrahedral intermediate then collapses, resulting in an H₂N-R₁ leaving group, which is protonated through His-57. Finally, His-57 deprotonates a water molecule, which can then serve as a nucleophile by similarly reacting with the carbonyl carbon. Collapse of the tetrahedral intermediate then results in a Ser-195 leaving group, which is protonated through His-57, resulting in all residues returned to their pre-catalytic state, and a carboxylic acid where there was previously a peptide bond.

Biological Function

Acrosin is the major proteinase present in the acrosome of mature spermatozoa. It is stored in the acrosome in its precursor form, proacrosin. Upon stimulus, the acrosome releases its contents onto the zona pellucida. After this reaction occurs, the zymogen form of the protease is then processed into its active form, β-acrosin. The active enzyme then functions in the lysis of the zona pellucida, thus facilitating penetration of the sperm through the innermost glycoprotein layers of the ovum.^[3]

The importance of acrosin in the acrosome reaction has been contested. It has been found through genetic knockout experiments that mouse spermatozoa lacking β-acrosin (the active protease) still have the ability to penetrate the zona pellucida.^[4] Thus, some argue for its role in assisting in the dispersal of acrosomal contents following the acrosome reaction, while others demonstrate evidence for its role as a secondary binding protein between the spermatozoa and zona pellucida.^[5]^[6]^[7] Under the secondary binding protein hypothesis, acrosin could serve a role in binding to molecules on the zona pellucida, tethering the spermatozoa to the egg. This "tethering" would ensure penetration due to the applied motile force of the spermatozoa.^[8]

Acrosin regulation has been found to occur through protein C inhibitor (PCI). PCI is present in the male reproductive tract at 40x higher concentrations than in blood plasma.^[9] PCI has been demonstrated to inhibit the proteolytic activity of acrosin.^[9] Thus, PCI has been hypothesized to have a protective role: if acrosomal enzymes were released prematurely, or if the spermatozoa was degenerated within the male reproductive tract, the high concentrations of PCI would inhibit acrosin from inflicting proteolytic damage on nearby tissues.^[10]

Structure

β-acrosin demonstrates a high degree of sequence identity (70-80%) between boar, bull, rat, guinea pig, mouse, and human isoforms.^[3] There exists a somewhat similar (27-35%) sequence identity between β-acrosin and other serine proteases such as trypsin and chymotrypsin.^[3] While most serine proteases are activated through one cleavage event, proacrosin requires processing at both the N and C-terminal domains. Proacrosin is first cleaved between Arg-22 and adjacent Valine to create a 22 residue light chain, and an active protease termed α-acrosin.^[3] This light chain remains associated with the heavy chain, cross-linked through two disulfide bonds to form a heterodimer. Following these N-terminal cleavage events, three cleavages at the C-terminal domain removes 70 residues, yielding β-acrosin.^[3] Acrosin has two sites which have been identified as possible N-glycosylation sites: Asn-2 and Asn-169.^[3]

The catalytic triad consists of residues His-57, Asp-102, and Ser-195.^[3] These residues are found in a binding pocket that has been termed the "S1" pocket, consistent with the naming scheme that has been adopted for other proteases.^[11] The S1 pocket regulates acrosin's specificity for Arg and Lys substrates, with a conserved Trp-215 serving as a "gatekeeper" residue for the binding site entrance.^[3]

An important structural element of β-acrosin is a highly charged patch (formed through both amino acids and post-translational modifications) on its surface region, that has been termed the "anion binding exosite."^[3] This site consists of an area of excess positive charge, which has been hypothesized to be important in binding to the matrix of the zona pellucida, a heavily glycosylated and sulfated region with excess negative charge.^[12] This structural feature is consistent with the secondary binding protein hypothesis, as charge-charge interactions would stabilize a protein-zona pellucida "tethering" complex.^[13] Further consistent with this structural hypothesis is the knowledge that suramin - a polysulfated drug (with substantial corresponding negative charge) has been found to inhibit sperm-zona pellucida binding.^[14]

Disease and Pharmaceutical Relevance

While one study which utilized mice models indicated that acrosin is not a necessary component of zona pellucida penetration, other studies in humans have shown an association between low acrosomal proteinase activity and infertility.^[15]^[16] Other research groups have demonstrated a significant correlation between acrosin activity and sperm motility.^[17] In rabbit models, an intravaginal contraceptive device that secreted tetradecyl sodium sulfate, a known inhibitor of acrosin and hyaluronidases, had a complete contraceptive effect.^[18] Although its exact mechanism of action is not entirely clear, acrosin could thus serve as a novel target for contraceptive agents. Acrosin may represent as a uniquely druggable target due to its location and high cellular specificity.^[19] Thus, developing inhibitors of acrosin could provide the basis for safe, reversible male contraceptives, or female contraceptives through the use of intravaginal contraceptive devices.^[19]

Moreover, as serine proteases are important in the potentiation of HIV, research has found that an acrosin inhibitor, 4'-acetamidophenyl 4-guanidinobenzoate, possess the ability to inhibit HIV infection in virus-inoculated lymphocytes.^[20] This suggests the further role of acrosin inhibitors as potentially viable agents in the prevention of HIV transmission.^[20]

References

^ Adham IM, Klemm U, Maier WM, Engel W (Jan 1990). "Molecular cloning of human preproacrosin cDNA". Human Genetics. 84 (2): 125–8. doi:10.1007/bf00208925. PMID 2298447. S2CID 39848902.
^ Honda A, Siruntawineti J, Baba T (2002). "Role of acrosomal matrix proteases in sperm-zona pellucida interactions". Human Reproduction Update. 8 (5): 405–12. doi:10.1093/humupd/8.5.405. PMID 12398221.
^ ^a ^b ^c ^d ^e ^f ^g ^h ⁱ ^j Tranter, Rebecca; Read, Jon A.; Jones, Roy; Brady, R. Leo (2000-11-15). "Effector Sites in the Three-Dimensional Structure of Mammalian Sperm β-Acrosin". Structure. 8 (11): 1179–1188. doi:10.1016/S0969-2126(00)00523-2. ISSN 0969-2126. PMID 11080640.
^ T. Baba, S. Azuma, S. Kashiwabara, Y. Toyoda. Sperm from mice carrying a targeted mutation of the acrosin gene can penetrate the oocyte zona pellucida and effect fertilization" J. Biol. Chem. 1994; 269 , pp. 31845–31849
^ K. Yamagata, T. Baba, et al. Acrosin accelerates the dispersal of sperm acrosomal proteins during acrosome reaction" J. Biol. Chem. 1998; 273 , pp. 10470–10474
^ R. Jones, C.R. Brown. Identification of a zona-binding protein from boar spermatozoa as proacrosin. Expl" Cell Res 1987; 171 , pp. 505–508
^ R. Jones. Interaction of zona pellucida glycoproteins, sulphated carbohydrates and synthetic polymers with proacrosin, the putative egg-binding protein from mammalian spermatozoa" Development 1991; 111 , pp. 1155–1163
^ D.P. Green. The head shapes of some mammalian spermatozoa and their possible relationship to the shape of the penetration slit through the zona pellucida. J. Reprod. Fertil., 83 (1988), pp. 377–387
^ ^a ^b Laurell, M; Christensson, A; Abrahamsson, PA; Stenflo, J; Lilja, H (1992). "Protein C inhibitor in human body fluids. Seminal plasma is rich in inhibitor antigen deriving from cells throughout the male reproductive system". J Clin Invest. 89 (4): 1094–101. doi:10.1172/JCI115689. PMC 442965. PMID 1372913.
^ Zheng, X; Geiger, M; Ecke, S (1994). "Inhibition of acrosin by protein C inhibitor and localization of protein C inhibitor to spermatozoa". Am. J. Physiol. 267 (2 Pt 1): C466–72. doi:10.1152/ajpcell.1994.267.2.C466. PMID 7521127.
^ I. Schechter, A. Berger. On the size of the active site in proteases. I. Papain. Biochim. Biophys. Res. Commun, 27 (1967), pp. 157–162.
^ Nakano M, Tobets T, et al. (1990). "Further fractionation of the glycoprotein families of porcine zona pellucida by anion exchange HPLC and some characterization of the separated fractions". J. Biochem. 107 (1): 144–150. doi:10.1093/oxfordjournals.jbchem.a122998. PMID 2110153.
^ S. Shimizu, M. Tsuji, J. Dean. In vitro biosynthesis of three sulphated glycoproteins of murine zonae pellucidae by oocytes grown in follicle culture" J. Biol. Chem. 1983; 258, pp. 5858–5863
^ Jones R, Parry R, Leggio LL, Nickel P (1996). "Inhibition of sperm-zona binding by suramin, a potential "lead" compound for design of new anti-fertility agents". Mol. Hum. Rep. 2 (8): 597–605. doi:10.1093/molehr/2.8.597. PMID 9239672.
^ Welker B, Bernstein GS, Diedrich K, Nakamura RM, Krebs D (Oct 1988). "Acrosomal proteinase activity of human spermatozoa and relation of results to semen quality". Hum Reprod. 3 (Suppl 2): 75–80. doi:10.1093/humrep/3.suppl_2.75. PMID 3068243.
^ Tummon I.S.; Yuzpe A.A.; Daniel S.A.; Deutsch A. Total acrosin activity correlates with fertility potential after fertilization in vitro" Fertil Steril 1991 Nov;56(5):933-8.
^ Cui YH, Zhao RL, Wang Q, Zhang ZY (Sep 2000). "Determination of sperm acrosin activity for evaluation of male fertility". Asian J Androl. 2 (3): 229–232. PMID 11225983.
^ Burck P.J., Zimmerman R.E. An intravaginal contraceptive device for the delivery of an acrosin and hyaluronidase inhibitor" Fertil Steril 1984 Feb;41(2):314-8.
^ ^a ^b Ning, Weiwei; Zhu, Ju; Zheng, Canhui; Liu, Xuefei; Song, Yunlong; Zhou, Youjun; Zhang, Xiaomeng; Zhang, Ling; Sheng, Chunquan (2013-04-01). "Fragment-Based Design of Novel Quinazolinon Derivatives as Human Acrosin Inhibitors". Chemical Biology & Drug Design. 81 (4): 437–441. doi:10.1111/cbdd.12106. ISSN 1747-0285. PMID 23331539. S2CID 21445655.
^ ^a ^b Bourinbaiar AS, Lee-Huang S (May 1995). "Acrosin inhibitor, 4'-acetamidophenyl 4-guanidinobenzoate, an experimental vaginal contraceptive with anti-HIV activity". Contraception. 51 (5): 319–22. doi:10.1016/0010-7824(95)00094-q. PMID 7628208.

External links

The MEROPS online database for peptidases and their inhibitors: S01.223
Acrosin at the U.S. National Library of Medicine Medical Subject Headings (MeSH)

This article incorporates text from the United States National Library of Medicine, which is in the public domain.

v t e Endopeptidases: serine proteases/serine endopeptidases (EC 3.4.21)
Digestive enzymes	Enteropeptidase Trypsin Chymotrypsin Elastase Neutrophil Pancreatic
Coagulation	factors: Thrombin Factor VIIa Factor IXa Factor Xa Factor XIa Factor XIIa Kallikrein PSA KLK1 KLK2 KLK3 KLK4 KLK5 KLK6 KLK7 KLK8 KLK9 KLK10 KLK11 KLK12 KLK13 KLK14 KLK15 fibrinolysis: Plasmin Plasminogen activator Tissue plasminogen activator Urinary plasminogen activator
Complement system	Factor B Factor D Factor I MASP MASP1 MASP2 C3-convertase
Other immune system	Chymase Granzyme Tryptase Proteinase 3/Myeloblastin
Venombin	Ancrod Batroxobin
Other	Acrosin Prolyl endopeptidase Pronase Proprotein convertases 1 2 Prostasin Reelin Subtilisin/Furin/S1P4 Sedolisin/TPP1 Streptokinase Cathepsin A G

v t e Enzymes
Activity	Active site Binding site Catalytic triad Oxyanion hole Enzyme promiscuity Diffusion-limited enzyme 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) EC7 Translocases (list)

This page was last edited on 30 December 2023, at 20:56

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