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THE IDENTIFICATION AND PURIFICATION OF A CELL‐SURFACE ALKALINE PHOSPHATASE FROM THE DINOFLAGELLATE PROROCENTRUM MINIMUM (DINOPHYCEAE) 1
Author(s) -
Dyhrman Sonya T.,
Palenik Brian P.
Publication year - 1997
Publication title -
journal of phycology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.85
H-Index - 127
eISSN - 1529-8817
pISSN - 0022-3646
DOI - 10.1111/j.0022-3646.1997.00602.x
Subject(s) - biology , dinoflagellate , alkaline phosphatase , biochemistry , dinophyceae , phosphate , centrifugation , differential centrifugation , size exclusion chromatography , chromatography , phosphatase , enzyme , botany , chemistry , phytoplankton , ecology , nutrient
Two cell‐surface proteins were identtjied in the dinoflagellate Prorocentrum minimum (Pavillard) Schilkr strain CCMP 1329 that are evident in phosphate‐limited cultures, but not in nitrate‐limited cultures or cultures growing exponentially in complete media. These proteins were detected by labeling cell‐surface proteins with the biotinylating reagent succinimidyl 6‐(biotinamido) hexanoate. One protein, of appoximately 200,000 daltons was purified using differential centrifugation, detergent extraction, and gel filtration chromatography. This purified protein was able to hydrolyze orthophosphate groups from p‐nitrophenylphosphate at pH 8, indicating it is an alkaline phosphatase, although it is larger than other alkaline phosphatases isolated to date tom most microorganisms. This protein may be induced to help P. minimum cleave orthophosphate groups from organic forms of phosphate in marine environments. Ultimately, this protein could represent a unique antigen for developing an antibody probe for examining the relationships between phosphate stress and bloom formation in P. minimum, and perhaps other dinoflagellates, in the field.