A FLOW PROCEDURE TO DETERMINE OXYGEN BINDING ISOTHERMS FOR LOW AFFINITY AND EASILY OXIDIZED HEMOGLOBINS

被引:9
作者
ASTATKE, M [1 ]
MCGEE, WA [1 ]
PARKHURST, LJ [1 ]
机构
[1] UNIV NEBRASKA,DEPT CHEM,LINCOLN,NE 68588
来源
COMPARATIVE BIOCHEMISTRY AND PHYSIOLOGY B-BIOCHEMISTRY & MOLECULAR BIOLOGY | 1992年 / 101卷 / 04期
关键词
D O I
10.1016/0305-0491(92)90359-Y
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
1. The determination of binding isotherms for low affinity hemoglobins is particularly difficult because of rapid autoxidation. 2. In carp Hb (pH 6 + IHP, 25-degrees-C), one-quarter of the hemes are oxidized within 3 min, preventing the accurate determination of even P50 or XBAR. 3. We circumvent this problem by rapidly flowing HbO2, initially at pH 9 (XBAR = 1.4 mu-M), against a low pH buffer to bring the system rapidly to equilibrium in the low affinity form. Diode-array spectrophotometry allows a complete spectrum to be obtained < 5 sec, after flow ceases, before significant oxidation has occurred. In tandem with the stopped flow apparatus in an oxygen electrode to measure O2 activity. 4. At 22-degrees-C, the half-saturation oxygen activity (XBAR) is 227-mu-M, and the Hill number is 0.91, for carp Hb (T state) implying significant differences in the O2 affinities of the alpha and beta chain hemes or, two different T states.
引用
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页码:683 / 688
页数:6
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