β-Galactosidase (EC 3.2.1.23, beta-gal or β-gal; systematic name β-D-galactoside galactohydrolase) is a glycoside hydrolase enzyme that catalyzes hydrolysis of terminal non-reducing β-D-galactose residues in β-D-galactosides. (This enzyme digests many β-Galactosides, not just lactose. It is sometimes loosely referred to as lactase but that name is generally reserved for mammalian digestive enzymes that breaks down lactose specifically.)
β-Galactosidase | |||||||||
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Identifiers | |||||||||
EC no. | 3.2.1.23 | ||||||||
CAS no. | 9031-11-2 | ||||||||
Databases | |||||||||
IntEnz | IntEnz view | ||||||||
BRENDA | BRENDA entry | ||||||||
ExPASy | NiceZyme view | ||||||||
KEGG | KEGG entry | ||||||||
MetaCyc | metabolic pathway | ||||||||
PRIAM | profile | ||||||||
PDB structures | RCSB PDB PDBe PDBsum | ||||||||
Gene Ontology | AmiGO / QuickGO | ||||||||
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galactosidase, beta 1 | |||||||
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Identifiers | |||||||
Symbol | GLB1 | ||||||
Alt. symbols | ELNR1 | ||||||
NCBI gene | 2720 | ||||||
HGNC | 4298 | ||||||
OMIM | 230500 | ||||||
RefSeq | NM_000404 | ||||||
UniProt | P16278 | ||||||
Other data | |||||||
Locus | Chr. 3 p22.3 | ||||||
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β-Galactosides include carbohydrates containing galactose where the glycosidic bond lies above the galactose molecule. Substrates of different β-galactosidases include ganglioside GM1, lactosylceramides, lactose, and various glycoproteins.[1]
Function
editβ-Galactosidase is an exoglycosidase which hydrolyzes the β-glycosidic bond formed between a galactose and its organic moiety. It may also cleave fucosides and arabinosides but at a much lower rate. It is an essential enzyme in the human body. Deficiencies in the protein can result in galactosialidosis or Morquio B syndrome. In E. coli, the lacZ gene is the structural gene for β-galactosidase; which is present as part of the inducible system lac operon which is activated in the presence of lactose when glucose level is low. β-Galactosidase synthesis stops when glucose levels are sufficient.[2]
β-Galactosidase has many homologues based on similar sequences. A few are evolved β-galactosidase (EBG), β-glucosidase, 6-phospho-β-galactosidase, β-mannosidase, and lactase-phlorizin hydrolase. Although they may be structurally similar, they all have different functions.[3] Beta-gal is inhibited by L-ribose and by competitive inhibitors 2-phenylethyl 1-thio-β-D-galactopyranoside (PETG), D-galactonolactone, isopropyl thio-β-D-galactoside (IPTG), and galactose.[4]
β-Galactosidase is important for organisms as it is a key provider in the production of energy and a source of carbons through the break down of lactose to galactose and glucose. It is also important for lactose-intolerant people as it is responsible for making lactose-free milk and other dairy products. Many adult humans lack the lactase enzyme, which has the same function as β-galactosidase, so they are not able to properly digest dairy products. β-Galactose is used in such dairy products as yogurt, sour cream, and some cheeses which are treated with the enzyme to break down any lactose before human consumption. In recent years, β-galactosidase has been researched as a potential treatment for lactose intolerance through gene replacement therapy where it could be placed into the human DNA so individuals can break down lactose on their own.[5][6]
Structure
editThe 1,023 amino acids of E. coli β-galactosidase were sequenced in 1983,[7] and its structure determined eleven years later in 1994. The protein is a 464-kDa homotetramer with 2,2,2-point symmetry.[8] Each unit of β-galactosidase consists of five domains; domain 1 is a jelly-roll type β-barrel, domain 2 and 4 are fibronectin type III-like barrels, domain 5 a novel β-sandwich, while the central domain 3 is a distorted TIM-type barrel, lacking the fifth helix with a distortion in the sixth strand.[8]
The third domain contains the active site.[9] The active site is made up of elements from two subunits of the tetramer, and disassociation of the tetramer into dimers removes critical elements of the active site. The amino-terminal sequence of β-galactosidase, the α-peptide involved in α-complementation, participates in a subunit interface. Its residues 22–31 help to stabilize a four-helix bundle which forms the major part of that interface, and residue 13 and 15 also contributing to the activating interface.[citation needed] These structural features provide a rationale for the phenomenon of α-complementation, where the deletion of the amino-terminal segment results in the formation of an inactive dimer.
Reaction
editβ-Galactosidase can catalyze three different reactions in organisms. In one, it can go through a process called transgalactosylation to make allolactose, creating a positive feedback loop for the production of β-galactose. Allolactose can also be cleaved to form monosaccharides. It can also hydrolyze lactose into galactose and glucose which will proceed into glycolysis.[3] The active site of β-galactosidase catalyzes the hydrolysis of its disaccharide substrate via "shallow" (nonproductive site) and "deep" (productive site) binding. Galactosides such as PETG and IPTG will bind in the shallow site when the enzyme is in "open" conformation while transition state analogs such as L-ribose and D-galactonolactone will bind in the deep site when the conformation is "closed".[4]
The enzymatic reaction consists of two chemical steps, galactosylation and degalactosylation. Galactosylation is the first chemical step in the reaction where Glu461 donates a proton to a glycosidic oxygen, resulting in galactose covalently bonding with Glu537. In the second step, degalactosylation, the covalent bond is broken when Glu461 accepts a proton, replacing the galactose with water. Two transition states occur in the deep site of the enzyme during the reaction, once after each step. When water participates in the reaction, galactose is formed, otherwise, when D-glucose acts as the acceptor in the second step, transgalactosylation occurs .[4] It has been kinetically measured that single tetramers of the protein catalyze reactions at a rate of 38,500 ± 900 reactions per minute.[10] Monovalent potassium ions (K+) as well as divalent magnesium ions (Mg2+) are required for the enzyme's optimal activity. The β-linkage of the substrate is cleaved by a terminal carboxyl group on the side chain of a glutamic acid.
In E. coli, Glu-461 was thought to be the nucleophile in the substitution reaction.[11] However, it is now known that Glu-461 is an acid catalyst. Instead, Glu-537 is the actual nucleophile,[12] binding to a galactosyl intermediate. In humans, the nucleophile of the hydrolysis reaction is Glu-268.[13] Gly794 is important for β-galactosidase activity. It is responsible for putting the enzyme in a "closed", ligand bounded, conformation or "open" conformation, acting like a "hinge" for the active site loop. The different conformations ensure that only preferential binding occurs in the active site. In the presence of a slow substrate, Gly794 activity increased as well as an increase in galactosylation and decrease in degalactosylation.[4]
Applications
editThe β-galactosidase assay is used frequently in genetics, molecular biology, and other life sciences.[14] An active enzyme may be detected using artificial chromogenic substrate 5-bromo-4-chloro-3-indolyl-β-D-galactopyranoside, X-gal. β-galactosidase will cleave the glycosidic bond in X-gal and form galactose and 5-bromo-4-chloro-3-hydroxyindole which dimerizes and oxidizes to 5,5'-dibromo-4,4'-dichloro-indigo, an intense blue product that is easy to identify and quantify.[15] It is used for example in blue white screen.[16] Its production may be induced by a non-hydrolyzable analog of allolactose, IPTG, which binds and releases the lac repressor from the lac operator, thereby allowing the initiation of transcription to proceed.
It is commonly used in molecular biology as a reporter marker to monitor gene expression. It also exhibits a phenomenon called α-complementation which forms the basis for the blue/white screening of recombinant clones. This enzyme can be split in two peptides, LacZα and LacZΩ, neither of which is active by itself but when both are present together, spontaneously reassemble into a functional enzyme. This property is exploited in many cloning vectors where the presence of the lacZα gene in a plasmid can complement in trans another mutant gene encoding the LacZΩ in specific laboratory strains of E. coli. However, when DNA fragments are inserted in the vector, the production of LacZα is disrupted, the cells therefore show no β-galactosidase activity. The presence or absence of an active β-galactosidase may be detected by X-gal, which produces a characteristic blue dye when cleaved by β-galactosidase, thereby providing an easy means of distinguishing the presence or absence of cloned product in a plasmid. In studies of leukaemia chromosomal translocations, Dobson and colleagues used a fusion protein of LacZ in mice,[17] exploiting β-galactosidase's tendency to oligomerise to suggest a potential role for oligomericity in MLL fusion protein function.[18]
A recent study conducted in 2020–2021 determined that Beta-Galactosidase activity correlates with senescence of the cells. Senescence of the cells can be interpreted as cells that do not divide, but cells that do not die. Beta-Galactosidase activity can be overexpressed, and this can lead to various diseases afflicting a wide range of body systems. These systems include the cardiovascular system, skeletal system, and many more. Detecting senescence cells can be achieved by measuring the lysosomal Beta-Galactosidase activity.[19]
A new isoform for beta-galactosidase with optimum activity at pH 6.0 (Senescence Associated beta-gal or SA-beta-gal) [20] which is specifically expressed in senescence (the irreversible growth arrest of cells). Specific quantitative assays were even developed for its detection.[21][15][22] However, it is now known that this is due to an overexpression and accumulation of the lysosomal endogenous beta-galactosidase,[23] and its expression is not required for senescence. Nevertheless, it remains the most widely used biomarker for senescent and aging cells, because it is reliable and easy to detect.
Evolution
editSome species of bacteria, including E. coli, have additional β-galactosidase genes. A second gene, called evolved β-galactosidase (ebgA) gene was discovered when strains with the lacZ gene deleted (but still containing the gene for galactoside permease, lacY), were plated on medium containing lactose (or other 3-galactosides) as sole carbon source. After a time, certain colonies began to grow. However, the EbgA protein is an ineffective lactase and does not allow growth on lactose. Two classes of single point mutations dramatically improve the activity of ebg enzyme toward lactose.[24][25] and, as a result, the mutant enzyme is able to replace the lacZ β-galactosidase.[26] EbgA and LacZ are 50% identical on the DNA level and 33% identical on the amino acid level.[27] The active ebg enzyme is an aggregate of ebgA -gene and ebgC-gene products in a 1:1 ratio with the active form of ebg enzymes being an α4 β4 hetero-octamer.[28]
Species distribution
editMuch of the work done on β-galactosidase is derived from E. coli. However the enzyme can be found in many plants (especially fruits), mammals, yeast, bacteria, and fungi.[29] β-galactosidase genes can differ in the length of their coding sequence and the length of proteins formed by amino acids.[30] This separates the β-galactosidases into four families: GHF-1, GHF-2, GHF-35, and GHF- 42.[31] E. Coli belongs to GHF-2, all plants belong to GHF-35, and Thermus thermophilus belongs to GHF-42.[31][30] Various fruits can express multiple β-galactosidase genes. There are at least seven β-galactosidase genes expressed in tomato fruit development, that have amino acid similarity between 33% and 79%.[32] A study targeted at identifying fruit softening of peaches found 17 different gene expressions of β-galactosidases.[30] The only other known crystal structure of β-galactosidase is from Thermus thermophilus. [31]
References
edit- ^ Dorland's Illustrated Medical Dictionary. Archived from the original on 2006-10-16. Retrieved 2006-10-22.
- ^ Garrett R (2013). Biochemistry. Belmont, CA: Cengage Learning. p. 1001. ISBN 978-1133106296.
- ^ a b "Glycoside hydrolase, family 1, β-glucosidase (IPR017736) < InterPro < EMBL-EBI". www.ebi.ac.uk. Retrieved 2015-12-11.
- ^ a b c d Juers DH, Hakda S, Matthews BW, Huber RE (November 2003). "Structural basis for the altered activity of Gly794 variants of Escherichia coli β-galactosidase". Biochemistry. 42 (46): 13505–11. doi:10.1021/bi035506j. PMID 14621996.
- ^ Salehi S, Eckley L, Sawyer GJ, Zhang X, Dong X, Freund JN, Fabre JW (January 2009). "Intestinal lactase as an autologous β-galactosidase reporter gene for in vivo gene expression studies". Human Gene Therapy. 20 (1): 21–30. doi:10.1089/hum.2008.101. PMID 20377368.
- ^ Ishikawa K, Kataoka M, Yanamoto T, Nakabayashi M, Watanabe M, Ishihara S, Yamaguchi S (July 2015). "Crystal structure of β-galactosidase from Bacillus circulans ATCC 31382 (BgaD) and the construction of the thermophilic mutants". The FEBS Journal. 282 (13): 2540–52. doi:10.1111/febs.13298. PMID 25879162. S2CID 33928719.
- ^ Kalnins A, Otto K, Rüther U, Müller-Hill B (1983). "Sequence of the lacZ gene of Escherichia coli". The EMBO Journal. 2 (4): 593–7. doi:10.1002/j.1460-2075.1983.tb01468.x. PMC 555066. PMID 6313347.
- ^ a b Jacobson RH, Zhang XJ, DuBose RF, Matthews BW (June 1994). "Three-dimensional structure of β-galactosidase from E. coli". Nature. 369 (6483): 761–6. Bibcode:1994Natur.369..761J. doi:10.1038/369761a0. PMID 8008071. S2CID 4241867.
- ^ Matthews BW (June 2005). "The structure of E. coli β-galactosidase". Comptes Rendus Biologies. 328 (6): 549–56. doi:10.1016/j.crvi.2005.03.006. PMID 15950161.
- ^ Juers DH, Matthews BW, Huber RE (December 2012). "LacZ β-galactosidase: structure and function of an enzyme of historical and molecular biological importance". Protein Science. 21 (12): 1792–807. doi:10.1002/pro.2165. PMC 3575911. PMID 23011886.
- ^ Gebler JC, Aebersold R, Withers SG (June 1992). "Glu-537, not Glu-461, is the nucleophile in the active site of (lac Z) β-galactosidase from Escherichia coli". The Journal of Biological Chemistry. 267 (16): 11126–30. doi:10.1016/S0021-9258(19)49884-0. PMID 1350782.
- ^ Yuan J, Martinez-Bilbao M, Huber RE (April 1994). "Substitutions for Glu-537 of β-galactosidase from Escherichia coli cause large decreases in catalytic activity". The Biochemical Journal. 299 (Pt 2): 527–31. doi:10.1042/bj2990527. PMC 1138303. PMID 7909660.
- ^ McCarter JD, Burgoyne DL, Miao S, Zhang S, Callahan JW, Withers SG (January 1997). "Identification of Glu-268 as the catalytic nucleophile of human lysosomal β-galactosidase precursor by mass spectrometry" (PDF). The Journal of Biological Chemistry. 272 (1): 396–400. doi:10.1074/jbc.272.1.396. PMID 8995274. S2CID 35101194.
- ^ Ninfa AJ, Ballou DP (2009). Fundamental Laboratory Approaches for Biochemistry and Biotechnology. ISBN 978-0-470-47131-9.
- ^ a b Gary RK, Kindell SM (August 2005). "Quantitative assay of senescence-associated beta-galactosidase activity in mammalian cell extracts". Analytical Biochemistry. 343 (2): 329–34. doi:10.1016/j.ab.2005.06.003. PMID 16004951.
- ^ β-Galactosidase Assay (A better Miller) - OpenWetWare
- ^ Dobson CL, Warren AJ, Pannell R, Forster A, Rabbitts TH (March 2000). "Tumorigenesis in mice with a fusion of the leukaemia oncogene Mll and the bacterial lacZ gene". The EMBO Journal. 19 (5): 843–51. doi:10.1093/emboj/19.5.843. PMC 305624. PMID 10698926.
- ^ Krivtsov AV, Armstrong SA (November 2007). "MLL translocations, histone modifications and leukaemia stem-cell development". Nature Reviews. Cancer. 7 (11): 823–33. doi:10.1038/nrc2253. PMID 17957188. S2CID 9183717.
- ^ Lozano-Torres, Beatriz; Blandez, Juan F.; Sancenón, Félix; Martínez-Máñez, Ramón (April 2021). "Chromo-fluorogenic probes for β-galactosidase detection". Analytical and Bioanalytical Chemistry. 413 (9): 2361–2388. doi:10.1007/s00216-020-03111-8. hdl:10251/180327. ISSN 1618-2642. PMID 33606064. S2CID 231957317.
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- ^ Bassaneze V, Miyakawa AA, Krieger JE (January 2008). "A quantitative chemiluminescent method for studying replicative and stress-induced premature senescence in cell cultures". Analytical Biochemistry. 372 (2): 198–203. doi:10.1016/j.ab.2007.08.016. PMID 17920029.
- ^ Itahana K, Campisi J, Dimri GP (2007). "Methods to Detect Biomarkers of Cellular Senescence". Biological Aging. Methods in Molecular Biology. Vol. 371. Humana Press. pp. 21–31. doi:10.1007/978-1-59745-361-5_3. ISBN 978-1-58829-658-0. PMID 17634571.
- ^ Lee BY, Han JA, Im JS, Morrone A, Johung K, Goodwin EC, et al. (April 2006). "Senescence-associated β-galactosidase is lysosomal β-galactosidase". Aging Cell. 5 (2): 187–95. doi:10.1111/j.1474-9726.2006.00199.x. hdl:2158/216175. PMID 16626397. S2CID 82432911.
- ^ Hall BG (January 1977). "Number of mutations required to evolve a new lactase function in Escherichia coli". Journal of Bacteriology. 129 (1): 540–3. doi:10.1128/JB.129.1.540-543.1977. PMC 234956. PMID 318653.
- ^ Hall BG (July 1981). "Changes in the substrate specificities of an enzyme during directed evolution of new functions". Biochemistry. 20 (14): 4042–9. doi:10.1021/bi00517a015. PMID 6793063.
- ^ Hall BG (October 1976). "Experimental evolution of a new enzymatic function. Kinetic analysis of the ancestral (ebg) and evolved (ebg) enzymes". Journal of Molecular Biology. 107 (1): 71–84. doi:10.1016/s0022-2836(76)80018-6. PMID 794482.
- ^ Stokes HW, Betts PW, Hall BG (November 1985). "Sequence of the ebgA gene of Escherichia coli: comparison with the lacZ gene". Molecular Biology and Evolution. 2 (6): 469–77. doi:10.1093/oxfordjournals.molbev.a040372. PMID 3939707.
- ^ Elliott AC, K S, Sinnott ML, Smith PJ, Bommuswamy J, Guo Z, et al. (February 1992). "The catalytic consequences of experimental evolution. Studies on the subunit structure of the second (ebg) β-galactosidase of Escherichia coli, and on catalysis by ebgab, an experimental evolvant containing two amino acid substitutions". The Biochemical Journal. 282 ( Pt 1) (1): 155–64. doi:10.1042/bj2820155. PMC 1130902. PMID 1540130.
- ^ Richmond ML, Gray JI, Stine CM (1981). "β-Galactosidase: Review of Recent Research Related to Technological Application, Nutritional Concerns, and Immobilization". Journal of Dairy Science. 64 (9): 1759–1771. doi:10.3168/jds.s0022-0302(81)82764-6. ISSN 0022-0302.
- ^ a b c Guo S, Song J, Zhang B, Jiang H, Ma R, Yu M (2018). "Genome-wide identification and expression analysis of β-galactosidase family members during fruit softening of peach [Prunus persica (L.) Batsch]". Postharvest Biology and Technology. 136: 111–123. doi:10.1016/j.postharvbio.2017.10.005.
- ^ a b c Rojas AL, Nagem RA, Neustroev KN, Arand M, Adamska M, Eneyskaya EV, et al. (November 2004). "Crystal structures of β-galactosidase from Penicillium sp. and its complex with galactose". Journal of Molecular Biology. 343 (5): 1281–92. doi:10.1016/j.jmb.2004.09.012. PMID 15491613.
- ^ Smith DL, Gross KC (July 2000). "A family of at least seven β-galactosidase genes is expressed during tomato fruit development". Plant Physiology. 123 (3): 1173–83. doi:10.1104/pp.123.3.1173. PMC 59080. PMID 10889266.
External links
edit- beta-Galactosidase at the U.S. National Library of Medicine Medical Subject Headings (MeSH)