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Inhibition of Alkaline Phosphatase from Pearl Oyster Pinctada fucata by o-Phthalaldehyde: Involvement of Lysine and Histidine Residues at the Active Site

Hongtao CHEN1Liping XIE1,2Zhenyan YU1Rongqing ZHANG1,2( )
Institute of Marine Biotechnology, Department of Biological Sciences and Biotechnology, Tsinghua University, Beijing 100084, China
Protein Science Laboratory of the Ministry of Education, Tsinghua University, Beijing 100084, China
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Abstract

Alkaline phosphatase from Pinctada fucata was inactivated by o-phthalaldehyde (OPA). The inactivation followed pseudo first-order kinetics with a second rate constant of 0.167 (mmol/L)-1 ·min-1 at pH 7.5 and 25℃. A Tsou's plot analysis showed that inactivation occurred upon formation of one isoindole group. The OPA-modified enzyme lost the ability to bind with the specific affinity column and the presence of substrates or competitive inhibitors protected the enzyme from inactivation. The results revealed that the OPA-reaction site was at the enzyme substrate binding site. Prior modification of the enzyme by lysine or histidine specific reagent abolished formation of the isoindole derivatives, suggesting that lysine and histidine residues were involved in the OPA-induced inactivation. Taken together, OPA inactivated the alkaline phosphatase from Pinctada fucata by cross-linking lysine and histidine residues at the active site and formed an isoindole group at the substrate binding site of the enzyme.

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Tsinghua Science and Technology
Pages 414-420

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Cite this article:
CHEN H, XIE L, YU Z, et al. Inhibition of Alkaline Phosphatase from Pearl Oyster Pinctada fucata by o-Phthalaldehyde: Involvement of Lysine and Histidine Residues at the Active Site. Tsinghua Science and Technology, 2005, 10(4): 414-420. https://doi.org/10.1016/S1007-0214(05)70092-4

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Received: 14 May 2004
Published: 01 August 2005
© Tsinghua University Press 2005