The interaction of recombinant subdomains of the procollagen C-proteinase with procollagen I provides a quantitative explanation for functional differences between the two splice variants, mammalian tolloid and bone morphogenetic protein 1.

6533b82afe1ef96bd128b9cb

RESEARCH PRODUCT

The interaction of recombinant subdomains of the procollagen C-proteinase with procollagen I provides a quantitative explanation for functional differences between the two splice variants, mammalian tolloid and bone morphogenetic protein 1.

Walter Stöcker Markus Höwel Vera Hintze Carsten Wermter Irene Yiallouros Eva Grosse Berkhoff Bernd Beermann Christoph Becker-pauly

subject

Proteases Protein Folding Tolloid-Like Metalloproteinases medicine.medical_treatment RNA Splicing Biology Antiparallel (biochemistry)Biochemistry Bone morphogenetic protein 1 law.invention Bone Morphogenetic Protein 1 law medicine Animals Protein precursor DNA Primers Protease Base Sequence Circular Dichroism Metalloendopeptidases Surface Plasmon Resonance Recombinant Proteins Procollagen peptidase Spectrometry Fluorescence Biochemistry Bone Morphogenetic Proteins Recombinant DNA Metalloproteases Electrophoresis Polyacrylamide Gel Astacin Procollagen

description

The procollagen C-proteinase (PCP) is a zinc peptidase of the astacin family and the metzincin superfamily. The enzyme removes the C-terminal propeptides of fibrillar procollagens and activates other matrix proteins. Besides its catalytic protease domain, the procollagen C-proteinase contains several C-terminal CUB modules (named after complement factors C1r and C1s, the sea urchin UEGF protein, and BMP-1) and EGF-like domains. The two major splice forms of the C-proteinase differ in their overall domain composition. The longer variant, termed mammalian tolloid (mTld, i.e., PCP-2), has the protease- CUB1-CUB2-EGF1-CUB3-EGF2-CUB4-CUB5 composition, whereas the shorter form termed bone morphogenetic protein 1 (BMP-1, i.e., PCP-1) ends after the CUB3 domain. Two related genes encode proteases similar to mTld in humans and have been termed mammalian tolloid like-1 and -2 (mTll-1 and mTll-2, respectively). For mTll-1, it has been shown that it has C-proteinase activity. We demonstrate that recombinant EGF1-CUB3, CUB3, CUB3-EGF2, EGF2-CUB4, and CUB4-CUB5 modules of the procollagen C-proteinase can be expressed in bacteria and adopt a functional antiparallel ‚-sheet conformation. As shown by surface plasmon resonance analysis, the modules bind to procollagen I in a 1:1 stoichiometry with dissociation constants (KD) ranging from 622.0 to 1.0 nM. Their binding to mature collagen I is weaker by at least 1 order of magnitude. Constructs containing EGF domains bind more strongly than those consisting of CUB domains only. This suggests that a combination of CUB and EGF domains serves as the minimal functional unit. The binding affinities of the EGF-containing modules for procollagen increase in the order EGF1-CUB3 < CUB3-EGF2 < EGF2-CUB4. In the context of the full length PCP, this implies that a given module has an affinity that continues to increase the more C-terminally the module is located within the PCP. The tightest binding module, EGF2-CUB4 (KD ) 1.0 nM), is only present in mTld, which might provide a quantitative explanation for the different efficiencies of BMP-1 and mTld in procollagen C-proteinase activity.

year	journal	country	edition	language
2006-05-24	Biochemistry

10.1021/bi060228k https://pubmed.ncbi.nlm.nih.gov/16716085