TY - JOUR
T1 - Characterization of glycated hemoglobin in diabetic patients
T2 - Usefulness of electrospray mass spectrometry in monitoring the extent and distribution of glycation
AU - Zhang, Xinyi
AU - Medzihradszky, Katalin F.
AU - Cunningham, John
AU - Lee, Phillip D.K.
AU - Rognerud, Cheryl L.
AU - Ou, Ching Nan
AU - Harmatz, Paul
AU - Witkowska, H. Ewa
N1 - Funding Information:
We are grateful to Dr. Cedric Shackleton for his support and expertise in mass spectrometric studies and to Dr. James Manning for his helpful discussion. This work was supported in part by the NIH Northern California Comprehensive Sickle Cell Center grant HL20985 and NIH grant M01RR01 271-19, Roche Vitamins (Parsippany, NJ, USA). The Micromass BioQ mass spectrometer was purchased from a grant of the NIH Shared Instrumentation Program (RR06505, C. Shackleton, PI). K.F.M. was supported by the NIH NCRR BRTP RR01614 (UCSF MS Facility, A.L. Burlingame, Director).
PY - 2001/8/5
Y1 - 2001/8/5
N2 - A combination of chromatographic and mass spectrometric techniques was used to evaluate the extent and distribution of glycation within the glycated hemoglobin (GHb) molecule. Studies on quantification of hemoglobin (Hb) glycation by electrospray ionization mass spectrometry (ES-MS) of intact globins employed specimens from 10 diabetic individuals and five normal controls. Detailed structural analysis of the phenylboronate affinity chromatography/ion-exchange (IE) HPLC-separated sub-populations of GHb was performed on a specimen carrying 13.7% GHb. An efficient protocol for mapping glycation sites within α and β globins was developed, e.g., Glu-C/Asp-N proteolytic digestion followed by LC-ES-MS. Relative site occupancy within discrete components of GHb was evaluated. A correlation between the degree of glycation measured at Hb level (by affinity chromatography) and at globin level (measured by ES-MS) was carried out. The above studies led us to conclude that during the process of phenylboronate chromatography GHb dimers, rather than tetramers, are bound to the affinity resin so a fraction of glycated dimers rather than tetramers is measured. This finding implies that a process of glycation affects a much higher number of native Hb tetramers than was previously contemplated. No glycation sites appear to be missed by phenylboronate affinity chromatography. We have found no evidence of the presence of multiple glycations within a single globin chain. While glycation of both globins within a dimer cannot be excluded, it is unlikely to be a significant phenomenon. According to ES-MS data, an equivalent of about one globin per αβ dimer of the affinity chromatography-isolated GHb carried glycation.
AB - A combination of chromatographic and mass spectrometric techniques was used to evaluate the extent and distribution of glycation within the glycated hemoglobin (GHb) molecule. Studies on quantification of hemoglobin (Hb) glycation by electrospray ionization mass spectrometry (ES-MS) of intact globins employed specimens from 10 diabetic individuals and five normal controls. Detailed structural analysis of the phenylboronate affinity chromatography/ion-exchange (IE) HPLC-separated sub-populations of GHb was performed on a specimen carrying 13.7% GHb. An efficient protocol for mapping glycation sites within α and β globins was developed, e.g., Glu-C/Asp-N proteolytic digestion followed by LC-ES-MS. Relative site occupancy within discrete components of GHb was evaluated. A correlation between the degree of glycation measured at Hb level (by affinity chromatography) and at globin level (measured by ES-MS) was carried out. The above studies led us to conclude that during the process of phenylboronate chromatography GHb dimers, rather than tetramers, are bound to the affinity resin so a fraction of glycated dimers rather than tetramers is measured. This finding implies that a process of glycation affects a much higher number of native Hb tetramers than was previously contemplated. No glycation sites appear to be missed by phenylboronate affinity chromatography. We have found no evidence of the presence of multiple glycations within a single globin chain. While glycation of both globins within a dimer cannot be excluded, it is unlikely to be a significant phenomenon. According to ES-MS data, an equivalent of about one globin per αβ dimer of the affinity chromatography-isolated GHb carried glycation.
KW - Glycated
KW - Hemoglobin
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U2 - 10.1016/S0378-4347(01)00196-7
DO - 10.1016/S0378-4347(01)00196-7
M3 - Article
C2 - 11499613
AN - SCOPUS:0035812225
SN - 1387-2273
VL - 759
SP - 1
EP - 15
JO - Journal of Chromatography B: Biomedical Sciences and Applications
JF - Journal of Chromatography B: Biomedical Sciences and Applications
IS - 1
ER -