An 1H-13C-13C-edited 1H NMR experiment for making resonance assignments in the active site of heme proteins

被引:10
|
作者
Qiu, F [1 ]
Rivera, M
Stark, RE
机构
[1] Oklahoma State Univ, Dept Chem, Stillwater, OK 74078 USA
[2] CUNY Coll Staten Isl, Dept Chem, Staten Isl, NY 10314 USA
[3] CUNY, Grad Sch, Staten Isl, NY 10314 USA
关键词
isotope editing; INEPT-INADEQUATE; double-quantum coherence; heme proteins; resonance assignments;
D O I
10.1006/jmre.1997.1276
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
In paramagnetic heme proteins, it is often problematic to make proton resonance assignments for heme substituents that do not have large isotropic shifts and consequently lie under the large envelope of polypeptide resonances. Furthermore, assignments that would normally be performed with the aid of HMBC experiments in diamagnetic molecules can prove difficult in the active site of paramagnetic heme proteins if T-2(-1) > (2)J(CH). To circumvent this problem, a new method is presented to selectively detect H-1 in H-1(n) - C-13 - C-13 fragments biosynthetically introduced into the active site of heme proteins. The pulse sequence combines well-known building blocks such as INEPT to transfer H-1 spin magnetization to bonded C-13 nuclei, followed by INADEQUATE to generate C-13 - C-13 double-quantum coherence that is selected with pulsed field gradients, and finally reverse-INEPT to transfer magnetization back to H-1 nuclei for subsequent observation. The new H-1(n) - C-13 - C-13 edited experiment takes advantage of the relatively large values of (1)J(CH) and (1)J(CC), avoiding the long interpulse delays in HMBC that compromise the detectability of rapidly relaxing nuclei. The potential applicability of the pulse sequence is demonstrated by its contribution to the unambiguous assignment of the carbonyl carbons in the heme propionates of ferricytochrome b(5). (C) 1998 Academic Press.
引用
收藏
页码:76 / 81
页数:6
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