
doi: 10.1271/bbb.60.1479
pmid: 8987597
As a first step in understanding the calcification mechanism, a matrix protein in the gastrolith of the crayfish Procambarus clarkii was purified and sequenced. The protein was insoluble in acid, but after trypsin digestion, it dissolved in 6 M urea. The trypsin-digested protein dissolved in urea solution was purified by reversed-phase HPLC and designated gastrolith matrix protein fragment. The fragment had a molecular weight of 9658 and a blocked amino terminus. It had tandemly repeated units not reported before at the central part of the sequence, with each unit being Gly-Ser-X1-X2-Phe as the most typical sequence. This peptide was found associated with chitin, a main component of the organic matrix.
Extracellular Matrix Proteins, Molecular Sequence Data, matrix protein, Astacoidea, Procambarus clarkii, chitin, Calculi, Peptide Fragments, Calcium Carbonate, calcification, Calcification, Physiologic, gastrolith, Animals, Amino Acid Sequence
Extracellular Matrix Proteins, Molecular Sequence Data, matrix protein, Astacoidea, Procambarus clarkii, chitin, Calculi, Peptide Fragments, Calcium Carbonate, calcification, Calcification, Physiologic, gastrolith, Animals, Amino Acid Sequence
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