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JBC, Vol. 253, Issue 7, 2327-2332, Apr, 1978
M. J. McDonald, R. Shapiro, M. Bleichman, J. Solway and H. F. Bunn
Human hemolysate contains several minor components designated Hb A1a, Hb
A1b, Hb A1c, which are post-translational modifications of the major
hemoglobin component A0. Individuals with diabetes mellitus have elevated
levels of Hb A1c, a hemoglobin modified with a glucose moiety at the NH2
terminus of each beta chain. A new chromatographic technique using Bio-Rex
70 is described which not only allows complete separation of Hb A1a from Hb
A1b but also resolution of Hb A1a into two components, designated Hb A1a1
and Hb A1a2. Carbohydrate determinations with the thiobarbituric acid
procedure revealed that Hb A1a1, Hb A1a2, and Hb A1b as well as Hb A1c were
glycosylated. Total phosphate analysis revealed 2.06 and 1.01 mol of
phosphorus/alphabeta dimer for Hb A1a1 and Hb A1a2 respectively; Hb A1b and
Hb A1c contained no detectable phosphate. Hemoglobin incubated with
D-[14C]glucose-6-P co-chromatographs precisely with Hb A1a2, strongly
suggesting that Hb A1a2 is glucose-6-P hemoglobin. Levels of Hb A1a1 and Hb
A1a2 are normal in individuals with diabetes mellitus. Furthermore,
diabetic red cells contain normal levels of glucose-6-P. Therefore,
glucose-6-P hemoglobin does not serve as a significant precursor to Hb A1c.
Instead Hb A1c is formed by the direct reaction of hemoglobin with glucose.
This suggests that hemoglobin can serve as a model system for nonenzymatic
glycosylation of protein.
Glycosylated minor components of human adult hemoglobin. Purification, identification, and partial structural analysis
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