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Entamoeba histolytica: an ecto-phosphatase activity regulated by oxidation-reduction reactions.

Experimental parasitology (2006-11-23)
Ana Acacia de Sá Pinheiro, Juliana Natal Amazonas, Fernanda de Souza Barros, Lúcia Feitosa De Menezes, Evander J O Batista, Edward Felix Silva, Wanderley De Souza, José Roberto Meyer-Fernandes
RESUMEN

In this work, an ecto-phosphatase activity of Entamoeba histolytica was characterized using intact cells. This activity presented the following biochemical characteristics: (i) it hydrolyzes p-NPP with V(max) of 8.00+/-0.22 nmol p-NP x h(-1) x 10(-5) cells and K(m) of 2.68+/-0.25 mM; (ii) it is inhibited by acid phosphatase inhibitors, such as sodium molybdate (K(i)=1.70+/-0.24 microM) and sodium fluoride (K(i)=0.25+/-0.02 mM); (iii) it also showed high sensitivity to phosphotyrosine phosphatase inhibitors, such as sodium orthovanadate (K(i)=1.07+/-0.14 microM), bpV-PHEN (K(i)=0.38+/-0.02 microM) and mpV-PIC (K(i)=0.39+/-0.04 microM). Zn(2+), an oxidizing agent, decreased the enzymatic activity in 50%. DTT and GSH, two reducing agents, enhanced the activity twofold. The non-invasive E. histolytica and free-living E. moshkovskii were less efficient in hydrolyzing p-NPP than the pathogenic E. histolytica suggesting that this enzyme could represent a virulence marker for this cell.

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Sodium molybdate dihydrate, ≥99.5%
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Sodium molybdate dihydrate, ACS reagent, ≥99%
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Sodium molybdate, ≥98%
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Sodium molybdate dihydrate, ≥99.5%, suitable for plant cell culture
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Sodium molybdate, anhydrous, powder, −100 mesh particle size, 99.9% trace metals basis
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Sodium molybdate dihydrate, 99.99% trace metals basis