Glial Cell Line-Derived Neurotrophic Factor:  Selective Reduction of the Intermolecular Disulfide Linkage and Characterization of Its Disulfide Structure

Haniu, Mitsuru; Hui, John O.; Young, Yunjen; Le, John C.; Katta, Viswanatham; Lee, Richard; Shimamoto, Grant; Rohde, Michael F.

doi:10.1021/bi9605550

Cited by 24 publications

(14 citation statements)

References 20 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…The cysteine adjacent to Cys-4 of the knot (Cys-X) played a pivotal role, since its mutation to alanine (construct pRMC-CXA) essentially prevented dimer formation. The Muc2-domaindimerization mechanism thus resembles that of TGF-β2 [25,26], vWF [28] and glial cell-line derived neurotrophic factor [27] in requiring this specific cysteine residue for dimer formation.…”

Section: Discussionmentioning

confidence: 94%

“…The Cys-X residue of monomeric TGF-β2 is reported to form a stable intermolecular disulphide bond with the equivalent cysteine in a second molecule of TGF-β2 [25,26]. The same residue is responsible for dimer formation of glial cell linederived neurotrophic factor [27]. Absence of this cysteine in the vWF polypeptide prevents dimerization, resulting in type IID von Willebrand disease [28] and mutagenesis of the same cysteine residue in norrin protein disrupts oligomer formation [29].…”

Section: Figure 1 Diagram Of the Cystine-knot Region Of Rmuc2mentioning

confidence: 99%

See 1 more Smart Citation

Role of the cystine-knot motif at the C-terminus of rat mucin protein Muc2 in dimer formation and secretion

Bell

Forstner

2001

Biochemical Journal

View full text Add to dashboard Cite

DNA constructs based on the 534-amino-acid C-terminus of rat mucin protein Muc2 (RMC), were transfected into COS cells and the resultant $&S-labelled dimers and monomers were detected by SDS\PAGE of immunoprecipitates. The cystine-knot construct, encoding the C-terminal 115 amino acids, appeared in cell lysates as a 45 kDa dimer, but was not secreted. A construct, devoid of the cystine knot, failed to form dimers. Site-specific mutagenesis within the cystine knot was performed on a conserved unpaired cysteine (designated Cys-X), which has been implicated in some cystine-knot-containing growth factors as being important for intermolecular disulphide-bond formation. Dimerization of RMC was effectively abolished. Each cysteine (Cys-1-Cys-6) comprising the three intramolecular disulphide bonds of the cystine knot was then mutated. Dimer formation

show abstract

Section: Discussionmentioning

confidence: 94%

Section: Figure 1 Diagram Of the Cystine-knot Region Of Rmuc2mentioning

confidence: 99%

Role of the cystine-knot motif at the C-terminus of rat mucin protein Muc2 in dimer formation and secretion

Bell

Forstner

2001

Biochemical Journal

View full text Add to dashboard Cite

show abstract

“…During or mucin polymerization and gel formation. Studies of dimer formashortly after N-glycosylation (presumably in the endoplasmic re-tion in transforming growth factor-β2 [14] and, more recently glial ticulum [41]), the monomers dimerized via disulphide bonds and cell line-derived neurotrophic factor [19], indicate that a likely gave a product having a mobility centred at 150 kDa.…”

Section: Metabolic Labeling and Immunoprecipitation Of Mucin Translatmentioning

confidence: 99%

“…The termed the 'cystine knot' motif, which is also present and plays protein core (or apomucin) usually consists centrally of a vari-an active role in the dimerization of transforming growth factorable number of imperfect tandem repeats which contribute to β2 [14], nerve-growth factor [15], Norrie disease protein [16, molecular rigidity because of extensive O-glycosylation of their 17], human chorionic gonadotropin [18] and glial cell line-deserine and threonine residues. The flanking end regions of most rived neurotrophic factor [19]. The involvement of the cystine secretory mucins are enriched in cysteine, contain consensus se-knot motif in the initial C-tail to C-tail dimerization of von Wilquences for N-glycosylation, and are presumed to be folded and lebrand factor has been documented using deletion mutants [20].…”

mentioning

confidence: 99%

Evidence that a peptide corresponding to the rat Muc2 C‐terminus undergoes disulphide‐mediated dimerization

Bell

Khatri

et al. 1998

European Journal of Biochemistry

View full text Add to dashboard Cite

We have investigated the possibility that the intestinal mucin rat Muc2 forms dimers during biosynthesis via intermolecular disulphide bridging of its C-terminal domains. Since the cysteine alignment of RMuc2 (and other secretory mucins) is similar to that of human von Willebrand factor, a similar C-tail to C-tail dimerization may occur in mucins. The C-terminal domain of RMuc2 (534 amino acids) was expressed in COS-1 cells, and the products monitored by SDS/PAGE and western blotting with three antibodies to different regions of the C-terminal domain. In cells, the expressed domain was glycosylated and formed disulphide-dependent dimers centred at approximately 150 kDa. The domain dimer, but not its precursor monomer, was secreted into the culture medium. The dimers in the media however, appeared to be 12Ϫ15-kDa heavier (i.e. had a slower mobility) than in cell lysates. Initial N-glycosylation, dimerization and secretion were inhibited by addition of tunicamycin to incubations, whereas benzyl-A-GalNAc did not interfere with these processes. However benzyl-A-GalNAc resulted in a decrease in the apparent size of secreted dimers, such that they now had the same mobility on gels as dimers normally seen in cell lysates (i.e. 150 kDa). A similar change in dimer size was observed after incubating untreated media samples with N-acetylneuraminidase. This suggests that benzyl-A-GalNAc caused inhibition of sialylation of cell dimers just before they were secreted. In summary, the C-terminal domain of RMuc2 can form disulphide-dependent dimers, and N-glycosylation is required for dimerization and subsequent secretion. A late sialylation event appears to precede the secretion of mucin domain dimers.Keywords : mucin ; Muc2; disulfide ; dimer; cystine knot.The internal epithelial surfaces of most organisms are cov-coprotein von Willebrand factor [6,8]. Other secretory mucins ered by a gel that is rich in secreted mucus glycoproteins (mu-show a similar cysteine distribution throughout their C-termini, cins). The gel lubricates the mucosal surface, forms a barrier to including frog integumentary mucin B.1 [9], bovine submaxilvarious chemicals, proteases, toxins and infectious agents, and is lary mucin [10], porcine submaxillary mucin [11] and human secreted in response to a wide variety of stimuli [1Ϫ4]. Several lung mucin MUC5AC [12,13]. The similarity includes a region domains of mucin molecules contribute to their function. The termed the 'cystine knot' motif, which is also present and plays protein core (or apomucin) usually consists centrally of a vari-an active role in the dimerization of transforming growth factorable number of imperfect tandem repeats which contribute to β2 [14], nerve-growth factor [15], Norrie disease protein [16, molecular rigidity because of extensive O-glycosylation of their 17], human chorionic gonadotropin [18] and glial cell line-deserine and threonine residues. The flanking end regions of most rived neurotrophic factor [19]. The involvement of the cystine secretory mucins are enriched in cystein...

show abstract

“…Complete Reduction with DTT and Alkylation with 4VP-The remaining disulfide bonds in partially reduced and alkylated VWF CK domains or purified fragments thereof were reduced with 50 mM DTT in 0.2 M Tris-HCl, pH 8.5, 6 M guanidine HCl, and alkylated with excess 4VP (21). The modified products were purified by RP-HPLC using a C18 column (2.1 ϫ 150 mm; Vydac/The Separation Group Inc.) and acetonitrile gradient.…”

mentioning

confidence: 99%

Localization of Disulfide Bonds in the Cystine Knot Domain of Human von Willebrand Factor

Katsumi

Tuley

Bodó

et al. 2000

Journal of Biological Chemistry

102

109

View full text Add to dashboard Cite

von Willebrand factor (VWF) is a multimeric glycoprotein that is required for normal hemostasis. After translocation into the endoplasmic reticulum, proVWF subunits dimerize through disulfide bonds between their C-terminal cystine knot-like (CK) domains. CK domains are characterized by six conserved cysteines. Disulfide bonds between cysteines 2 and 5 and between cysteines 3 and 6 define a ring that is penetrated by a disulfide bond between cysteines 1 and 4. Dimerization often is mediated by additional cysteines that differ among CK domain subfamilies. When expressed in a baculovirus system, recombinant VWF CK domains (residues 1957-2050) were secreted as dimers that were converted to monomers by selective reduction and alkylation of three unconserved cysteine residues: Cys 2008 , Cys

show abstract

Glial Cell Line-Derived Neurotrophic Factor: Selective Reduction of the Intermolecular Disulfide Linkage and Characterization of Its Disulfide Structure

Cited by 24 publications

References 20 publications

Role of the cystine-knot motif at the C-terminus of rat mucin protein Muc2 in dimer formation and secretion

Role of the cystine-knot motif at the C-terminus of rat mucin protein Muc2 in dimer formation and secretion

Evidence that a peptide corresponding to the rat Muc2 C‐terminus undergoes disulphide‐mediated dimerization

Localization of Disulfide Bonds in the Cystine Knot Domain of Human von Willebrand Factor

Contact Info

Product

Resources

About