Familial cases of point mutations in the XIST promoter reveal a correlation between CTCF binding and pre-emptive choices of X chromosome inactivation

A specific and sensitive "sandwich"-type enzyme-linked immunosorbent assay (ELISA) has been developed for quantifying human apo A-IV. Using apo A-IV immunosorbent columns, we isolated monospecific anti-apo A-IV antibodies for coating the ELISA plates and for preparing peroxidase-antibody conjugate. The assay can detect as little as 0.20 ng of apo A-IV, with mean intra- and interassay CVs of 3.6% and 8.2%, respectively. The apoA-IV concentrations in normolipemic and hyperlipemic plasma were unaffected by either delipidation or treatment with detergents or urea. To validate the ELISA assay we compared it with an immunoelectrophoretic technique. ApoA-IV concentrations in plasma from normo- and dyslipemic subjects compared well by the two assays (r = 0.89). The mean apo A-IV concentration, measured by ELISA in plasma from 50 normolipemic subjects, was 143 (SD 52) mg/L; values for dyslipemic subjects were not significantly different. We also used this new assay to monitor apo A-IV profiles of normolipemic and hypertriglyceridemic plasma after chromatographic fractionation.

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Subcellular distribution of androgens in hyperplastic human prostate

Verdonck¹,

Slypere

Moussa³

et al. 1980

Journal of Steroid Biochemistry

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J.P. De Slypere

Normal reference values for creatine, creatinine, and carnitine are lower in vegetarians.

Pseudohypertriglyceridemia due to benign glycerol kinase deficiency

Quantification of human apolipoprotein A-IV by "sandwich"-type enzyme-linked immunosorbent assay.

Subcellular distribution of androgens in hyperplastic human prostate

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