Procollagen N-proteinase. Properties of the enzyme purified from chick embryo tendons. Academic Article

abstract

• Procollagen N-proteinase was purified about 3700-fold from chick embryo tendons. Electrophoresis of the protein after iodination and denaturation suggested it was homogeneous. However, the native enzyme could not be examined by gel electrophoresis, and therefore homogeneity of the preparation was not conclusively established. Antibodies to the enzyme completely inhibited activity and gave a single precipitant line by double immuno-diffusion. The Km for a native procollagen substrate was 0.3-0.5 microM. The same protein after denaturation inhibited activity. The enzyme did not cleave type III procollagen from human fibroblasts or a type IV procollagen from a mouse sarcoma. Ca2+ was required for maximal enzymic activity. The data suggested a second metal requirement, but this was not identified. Reducing agents and metal chelators inhibited activity, but there was little if any inhibition from several inhibitors of other neutral metalloproteinases.

authors

• Prockop, Darwin

published proceedings

• Eur J Biochem

altmetric score

• 3

author list (cited authors)

• Tuderman, L., & Prockop, D. J.

citation count

• 62

complete list of authors

• Tuderman, L||Prockop, DJ

publication date

• July 1982

publisher

• Wiley  Publisher

published in

• European Journal of Biochemistry  Journal

keywords

• Animals
• Chelating Agents
• Chick Embryo
• Collagen
• Endopeptidases
• Iodine Radioisotopes
• Metals
• Procollagen
• Procollagen N-Endopeptidase
• Protease Inhibitors
• Rabbits
• Tendons

PubMed Central ID

• 6811269

Digital Object Identifier (DOI)

• 10.1111/j.1432-1033.1982.tb06716.x

start page

• 545

end page

• 549

volume

• 125

issue

• 3

URL

• http://dx.doi.org/10.1111/j.1432-1033.1982.tb06716.x