Literature DB >> 3009301

Phenotypic variation in the phosphotransferase activity of human red cell acid phosphatase (ACP1).

V L Golden, G F Sensabaugh.   

Abstract

Red cell acid phosphatase (ACP1) catalyses the transfer of phosphate from phosphate ester substrates to suitable acceptor alcohols such as methanol and glycerol. The rate of substrate turnover in the presence of acceptors is increased by the increment of the phosphotransferase reaction, thus allowing this activity to be measured. There is specificity with regard to acceptors: (a) polyols (e.g., glycerol) are better acceptors than the corresponding n-alcohols, and (b) polyol configuration and chain length determine acceptor activity. Ribitol was the most efficient acceptor found. Each of the three common ACP1 alleles is represented electrophoretically by two isozyme bands; the phosphotransferase activity of the anodal isozyme was found to be more than twice that of the cathodal isozyme. The extent of phosphotransferase activity is also genotype dependent. In the presence of 2 M glycerol, the relative phosphotransferase efficiencies for the three homozygote types were: ACP1 B = 3.7, ACP1 A = 3.4, and ACP1 C = 2.5. This pattern of B greater than A greater than C is the same as found for the modulation of ACP1 by purines and folates.

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Year:  1986        PMID: 3009301     DOI: 10.1007/bf00290961

Source DB:  PubMed          Journal:  Hum Genet        ISSN: 0340-6717            Impact factor:   4.132


  17 in total

1.  GENETICAL STUDIES ON HUMAN RED CELL ACID PHOSPHATASE.

Authors:  D A HOPKINSON; N SPENCER; H HARRIS
Journal:  Am J Hum Genet       Date:  1964-03       Impact factor: 11.025

2.  Methods for the isolation of glycolytic intermediated by column chromatography with ion exchange resins.

Authors:  G R BARTLETT
Journal:  J Biol Chem       Date:  1959-03       Impact factor: 5.157

3.  Human red cell glycolytic intermediates.

Authors:  G R BARTLETT
Journal:  J Biol Chem       Date:  1959-03       Impact factor: 5.157

4.  Standardization of hemoglobinometry. II. The hemiglobincyanide method.

Authors:  E van KAMPEN; W G ZIJLSTRA
Journal:  Clin Chim Acta       Date:  1961-07       Impact factor: 3.786

5.  Activation of low molecular weight acid phosphatase from bovine brain by purines and glycerol.

Authors:  M M Tanizaki; H M Bittencourt; H Chaimovich
Journal:  Biochim Biophys Acta       Date:  1977-11-23

6.  Activity of the "red cell" acid phosphatase locus in other tissues.

Authors:  D M Swallow; S Povey; H Harris
Journal:  Ann Hum Genet       Date:  1973-07       Impact factor: 1.670

7.  Human erythrocytic acid phosphatase: resolution and characterization of the isozymes from three homozygous phenotypes.

Authors:  M R Fenton; K E Richardson
Journal:  Arch Biochem Biophys       Date:  1971-01       Impact factor: 4.013

8.  A comparison of some properties of human red cell acid phosphatase in different phenotypes.

Authors:  J E Luffman; H Harris
Journal:  Ann Hum Genet       Date:  1967-05       Impact factor: 1.670

9.  Phenotypic differences in purine modulation of erythrocyte acid-phosphatase activity.

Authors:  E Mansfield; G F Sensabaugh
Journal:  Lancet       Date:  1977-07-23       Impact factor: 79.321

10.  Phenotype dependence in the inhibition of red cell acid phosphatase (ACP) by folates.

Authors:  G F Sensabaugh; V L Golden
Journal:  Am J Hum Genet       Date:  1978-09       Impact factor: 11.025

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  2 in total

1.  Human red cell acid phosphatase (ACP1): evidence for differences in the primary structure of the two isozymes encoded by the ACP1*B allele.

Authors:  J Dissing; G F Sensabaugh
Journal:  Biochem Genet       Date:  1987-12       Impact factor: 1.890

2.  A possible genetic component of obesity in childhood. Observations on acid phosphatase polymorphism.

Authors:  N Lucarini; G Finocchi; F Gloria-Bottini; M Macioce; P Borgiani; A Amante; E Bottini
Journal:  Experientia       Date:  1990-01-15
  2 in total

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