Proglyprot

ProGP101 (H(A16-M) (1,3-1,4)-beta-glucanase)

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ProGP ID	ProGP101 (H(A16-M) (1,3-1,4)-beta-glucanase)
Validation Status	Characterized
Organism Information
Organism Name	Paenibacillus (Bacillus) macerans and Bacillus amyloliquefaciens (velezensis)
Domain	Bacteria
Classification	Phylum : Firmicutes Class : Bacilli Orders : Bacillales Family : Paenibacillaceae Genus : Paenibacillus Species : macerans
Taxonomic ID (NCBI)	44252
Genome Information
GenBank	X55959
EMBL	X55959
Protein Information
Protein Name	H(A16-M) (1,3-1,4)-beta-glucanase
UniProtKB/SwissProt ID	P23904
EMBL-CDS	CAA39426.1
UniProtKB Sequence	>sp\|P23904\|GUB_PAEMA Beta-glucanase OS=Paenibacillus macerans PE=1 SV=2 MKKKSCFTLVTTFAFSLIFSVSALAGSVFWEPLSYFNRSTWEKADGYSNGGVFNCTWRAN NVNFTNDGKLKLGLTSSAYNKFDCAEYRSTNIYGYGLYEVSMKPAKNTGIVSSFFTYTGP AHGTQWDEIDIEFLGKDTTKVQFNYYTNGVGGHEKVISLGFDASKGFHTYAFDWQPGYIK WYVDGVLKHTATANIPSTPGKIMMNLWNGTGVDDWLGSYNGANPLYAEYDWVKYTSN
Sequence length	237 AA
Subcellular Location	Secreted
Function	It is the hybrid enzyme that catalyses cleavage of (1,4)-beta-linkages of O-substituted beta-D-glucanopyranosyl residues.
Protein Structure
PDB ID	1CPM, 1GLH, 2AYH
Glycosylation Status
Glycosylation Type	N- (Asn) linked
Experimentally Validated Glycosite(s) in Full Length Protein	(Signal peptide: 1-25) N56, N210
Experimentally Validated Glycosite(s ) in Mature Protein	N31, N185
Glycosite(s) Annotated Protein Sequence	MKKKSCFTLVTTFAFSLIFSVSALAQTGGSFFEPFNSYNSGTWEKADGYSNGGVFN(56)CTWR ANNVNFTNDGKLKLGLTSSAYNKFDCAEYRSTNIYGYGLYEVSMKPAKNTGIVSSFFTYT GPAHGTQWDEIDIEFLGKDTTKVQFNYYTNGVGGHEKVISLGFDASKGFHTYAFDWQPGY IKWYVDGVLKHTATANIPSTPGKIMMNLWN(210)GTGVDDWLGSYNGANPLYAEYDWVKYTSN This sequence has 16 N-terminal amino acids (colored red) derived from AMY. The remaining residues are from MAC.
Sequence Around Glycosites (21 AA)	ADGYSNGGVFNCTWRANNVNF TPGKIMMNLWNGTGVDDWLGS
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Technique(s) used for Glycosylation Detection	Mass shift detected after deglycosylation with Endo Hf and PNGase F
Technique(s) used for Glycosylated Residue(s) Detection	N-terminal sequencing
Protein Glycosylation- Implication	There is a large influence of N glycosylation on the thermostability of the hybrid enzyme. 16- and 133-fold decrease of thermostability has been observed after treatment with endoglycosidase H and peptide:N-glycosidase F (that remove glycans). This indicates that N-glycans are a major determinant for the resistance of this hybrid glucanase to thermal inactivation.
Glycan Information
Glycan Annotation	Linkage: GlcNAc-N-Asn
Protein Glycosylation linked (PGL) gene(s)
Additional Comment	Engineered glycoprotein The glucanases from which the hybrid enzyme is made, are not glycosylated in their native hosts. Hybrid enzyme containing 16 N-terminal amino acids from Bacillus amyloliquefaciens (1,3-1,4)-beta-glucanase (AMY), and remaining C-terminal part and signal peptide from B. macerans (1,3-1,4)-beta-glucanase (MAC), was expressed in Saccharomyces cerevisiae to see the effect of N-glycosylation on the thermostability of the hybrid enzyme. Information from UniProtKB and EMBL has been provided for MAC enzyme as it constitutes the major part of the hybrid enzyme (239 AA). UniProtKB ID for AMY is P07980.
Literature
Year of Identification	1994
Year of Identification Month Wise	1994.01.01
Year of Validation	1994
Reference	Hahn, M., Keitel, T. and Heinemann, U., 1995. Crystal and Molecular Structure at 0.16‐nm Resolution of the Hybrid Bacillus Endo‐1, 3‐1, 4‐β‐D‐Glucan 4‐Glucanohydrolase H (A16‐M). European journal of biochemistry, 232(3), pp.849-858.
Contact	Research group crystallography, Max Delbrück Center for Molecular Medicine, Berlin, Germany.
Reference	Meldgaard, M., 1994. Different effects of N-glycosylation on the thermostability of highly homologous bacterial (1, 3-1, 4)-β-glucanases secreted from yeast. Microbiology, 140(1), pp.159-166.
Corresponding Author	M Meldgaard
Contact	Department of Physiology, Carlsberg Laboratory, Copenhagen, Denmark.
Reference	Hahn, M., Piotukh, K., Borriss, R. and Heinemann, U., 1994. Native-like in vivo folding of a circularly permuted jellyroll protein shown by crystal structure analysis. Proceedings of the National Academy of Sciences, 91(22), pp.10417-10421.
Contact	Research group crystallography, Max Delbrück Center for Molecular Medicine, Berlin, Germany.
Reference	Keitel, T., Meldgaard, M. and Heinemann, U., 1994. Cation binding to a Bacillus (1, 3–1, 4)‐β‐glucanase Geometry, affinity and effect on protein stability. European Journal of Biochemistry, 222(1), pp.203-214.
Corresponding Author	Udo Heinemann
Contact	Institute of Crystallography, Freie Universität Berlin, Germany
Reference	Olsen, O. and Thomsen, K.K., 1991. Improvement of bacterial β-glucanase thermostability by glycosylation. Microbiology, 137(3), pp.579-585.
Corresponding Author	Karl Kristian Thomsen
Contact	Carlsberg Laboratory, Department of Physiology, Gamle Carlsbergvej 10, DK-2500 Copenhagen Valby, Denmark