Dual-isotope separation technique for radioassay of Cobalamin
Cobalamin is assayed by a dual-isotope separation method using sodium [ 125I]iothalamate as a marker. Two systems are used: one in which the incompletely-separated bound fraction is counted and compared with the single-isotope method in which the bound fraction is separated by washing (Phadebas radi...
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Veröffentlicht in: | Clinica chimica acta 1979, Vol.91 (1), p.23-39 |
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Format: | Artikel |
Sprache: | eng |
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Zusammenfassung: | Cobalamin is assayed by a dual-isotope separation method using sodium [
125I]iothalamate as a marker. Two systems are used: one in which the incompletely-separated bound fraction is counted and compared with the single-isotope method in which the bound fraction is separated by washing (Phadebas radiosorbent assay); and one in which an aliquot of the free fraction is counted.
In the dual-isotope method counting bound fractions, about 97% of the supernatant is removed by pouring from silicone fluid separators. The results for serum samples obtained using dual- and single-isotope methods were similar (between run coefficients of variation 5–7%). Experimental errors were smaller in the dual-isotope method.
A factor in the kit standards, presumably the absence of proteins, was found to affect the separation technique, resulting in relatively large experimental errors for standards in the single-isotope method. Washing the solid phase in the single-isotope method apparently resulted in a loss of bound isotope.
In the dual-isotope method counting free fractions reasonable precision was obtained (coefficient of variation of serum samples 6.6%) even though only about 56% of the supernatant (free fraction) was counted. |
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ISSN: | 0009-8981 1873-3492 |
DOI: | 10.1016/0009-8981(79)90467-4 |