Your search keyword '"Wajcman H"' showing total 23 results

1. Detection of neutral and charged mutations in alpha- and beta-human globin chains by capillary zone electrophoresis in isoelectric, acidic buffers.

Author

Saccomani A, Gelfi C, Wajcman H, and Righetti PG

Subjects

Buffers, Electrophoresis, Capillary, Erythrocytes chemistry, Globins isolation & purification, Humans, Indicators and Reagents, Isoelectric Focusing, Globins genetics, Mutation physiology

Abstract

A simple and reliable method, for screening for point mutations in alpha- and beta-human globin chains, is reported here, utilizing capillary zone electrophoresis in isoelectric, acidic buffers. A solution of 50 mM iminodiacetic acid (pI 2.23) containing 7 M urea and 0.5% hydroxyethylcellulose (apparent pH 3.2) is used as background electrolyte for fast separation of heme-free, denatured globin (alpha and beta) chains. Due to the low conductivity of such buffers, high voltage gradients (600 V/cm) can be applied, thus reducing the separation time to only a few minutes. In presence of neutral to neutral amino acid substitutions, it is additionally shown that the inclusion of 3% surfactant (Tween 20) in the sample and background electrolyte induces the separation of the wild-type and mutant chains, probably by a mechanism of hydrophobic interaction of the more hydrophobic mutant with the detergent micelle, via a mechanism similar to "micellar electrokinetic chromatography". At this low operative pH, however, charged mutants, involving substitutions of acidic amino acids (Glu and Asp) are not detected, since these residues are extensively protonated. Curiously, however, they are still separated in presence of detergent, due to the large variation in hydrophobicity involved in such mutations. Of the 19 mutants analyzed, all but one were resolved: Hb St Nazaire (beta 103 Phe-->Ile). This is due to the fact that the delta G (in kcal/mol) in the substitution Phe-->Ile is zero, thus no separation can possibly take place between two chains exhibiting the same hydrophobicity parameter.

Published

1999

2. Generation of tryptic maps of alpha- and beta-globin chains by capillary electrophoresis in isoelectric buffers.

Author

Capelli L, Stoyanov AV, Wajcman H, and Righetti PG

Subjects

Adult, Amino Acid Sequence, Buffers, Hemoglobins classification, Hemoglobins metabolism, Humans, Hydrogen-Ion Concentration, Molecular Sequence Data, Peptide Fragments chemistry, Peptide Mapping, Trypsin metabolism, Chromatography, High Pressure Liquid methods, Electrophoresis, Capillary methods, Hemoglobins isolation & purification, Peptide Fragments analysis

Abstract

A novel method for generating peptide maps, following tryptic digests of proteins, is reported here: capillary zone electrophoresis in the presence of isoelectric buffers as the sole buffering species. A typical buffer composition comprises 50 mM aspartic acid (pH = pI = 2.77), 0.5% hydroxyethyl cellulose (added as a dynamic coating agent for preventing peptide adsorption to weakly ionized silanols), 5% trifluoroethanol and 1% zwitterionic detergent (CHAPS). With this buffer composition, a high-voltage gradient can be applied (typically 600 V/cm in 75 microns I.D. and 900 V/cm in 50 microns I.D. capillaries), thus drastically reducing the analysis times. The method is applied to the generation of peptide maps of alpha- and beta-globin chains from human adult hemoglobin. In the case of beta-peptides, at an operative pH of 2.77, which represents a cross-over point in the titration curve of peptides T2 and T9, the two analytes merge into a single peak. However it is shown that it is possible to change the pH of the zwitterionic buffer by adjusting its concentration in solution. In 30 mM Asp (pH 3.0) or 20 mM Asp (pH 3.1) resolution of these two peptides is fully restored. Isoelectric, amphoteric buffers thus seem to represent a novel, powerful buffer system able to offer high resolution and high selectivity.

Published

1997

3. Perfusion chromatography on reversed-phase column allows fast analysis of human globin chains.

Author

Wajcman H, Ducrocq R, Riou J, Mathis M, Godart C, Prehu C, and Galacteros F

Subjects

Chromatography, Humans, Perfusion, Hemoglobins analysis

Abstract

Human globin chain analysis provides important information on the genetics and molecular pathophysiology of hemoglobinopathies. We propose using perfusion chromatography on the reversed-phase stationary phase to perform these studies. The technique, herein described, involves a high-velocity flow of the mobile phase through a porous chromatographic stationary phase made of microspheres of poly(styrene-divinylbenzene) having throughpores of 6000-8000 A diameter with short diffusive pores of 500-1000 A diameter connected to them. The composition of fetal hemoglobin (Ggamma:Agamma ratio) is determined, using this method, as an order of magnitude faster than with conventional HPLC. Elution is performed by developing a linear gradient of acetonitrile at a flow rate of 3 ml/min (or more), easily obtained on any HPLC machine. Analyses may be done on samples containing as low as 3.0% Hb F. Results are similar to those obtained with the reference HPLC technique, which uses a C4 column. In addition, reversed-phase perfusion chromatography, using a shallow curvilinear gradient, may help in the characterization of Hb variants. This technique allowed us to discriminate several alpha and beta chain mutants from variants that have closely similar patterns of electrophoretic mobilities.

Published

1996

4. Perfusion chromatography allows an order of magnitude faster measurement of the G gamma: A gamma ratio in patients with an increased level of fetal hemoglobin.

Author

Wajcman H, Galacteros F, and Ducrocq R

Subjects

Humans, Perfusion, Chromatography methods, Fetal Hemoglobin analysis, Globins analysis

Published

1996

5. Geographic distribution of 119 alleles of the alpha and beta globin genes detected in 432 French Caucasian carriers of haemoglobin variant.

Author

Chami B, Braconnier F, Riou J, Bardakdjian-Michau J, Préhu C, Blouquit Y, Rosa J, Wajcman H, and Galactéros F

Subjects

Alleles, France, Gene Frequency, Humans, Point Mutation, White People, Globins genetics, Hemoglobins, Abnormal genetics

Abstract

The French population is the result of mixing of different peoples including the Celts, Saxons, Germans, Italians and Hispanics. Between 1981 and 1993 patients were selected during investigations in France for haematological disorders associated or otherwise with the presence of a haemoglobin (Hb) variant. Further carriers of abnormal Hb were identified by HPLC measurement of glycated Hb in diabetics and by neonatal screening. Four-hundred and thirty-two subjects were found to be heterozygous for one of the 119 different alpha and the beta gene alleles encountered. These variants were characterised by a combination of 6 electrophoretic methods and in some cases by protein structure determinations. Some mutants reflected the population movements in and into France. A few mutants are frequently described in the French Caucasian population: Hb Lepore Boston, Hb D Punjab, whereas others appear to be anthropological markers. Hb Winnipeg has only been found in the West of France (Normandy); Hb J Baltimore is mainly found in French subjects of Spanish origin. Several cases of sporadic and previously undescribed mutations of Hb were identified. The last immigration waves from Africa and Asia appear to have contributed to the evolution of the pattern of haemoglobinopathies in the French population (Hb S, Hb O Arab or Hb C).

Published

1995

6. Heme binding to calmodulin, troponin C, and parvalbumin, as a probe of calcium-dependent conformational changes.

Author

Leclerc E, Leclerc L, Cassoly R, der Terrossian E, Wajcman H, Poyart C, and Marden MC

Subjects

Animals, Brain metabolism, Calmodulin chemistry, Carbon Monoxide, Cattle, Chromatography, High Pressure Liquid, Intercellular Signaling Peptides and Proteins, Kinetics, Muscles metabolism, Parvalbumins chemistry, Peptide Fragments isolation & purification, Peptides, Protein Binding, Spectrometry, Fluorescence, Spectrophotometry, Troponin chemistry, Troponin C, Wasp Venoms metabolism, Calcium pharmacology, Calmodulin metabolism, Heme metabolism, Parvalbumins metabolism, Protein Conformation, Troponin metabolism

Abstract

Heme-CO binds to the active (calcium-bound) form of calmodulin (CaM), but not to the inactive form. Despite a similarity in structure of another calcium-binding protein, skeletal muscle troponin C, both the affinity and the spectral red-shift of the absorption of the heme group are greatly decreased for troponin C relative to calmodulin. Parvalbumin, another calcium-binding protein, shows a twofold greater affinity for heme-CO relative to CaM. Unlike calmodulin and troponin C, the affinity of parvalbumin for heme-CO is even greater in the absence of calcium. The affinity of the tryptic and thrombic fragments of CaM for heme-CO are decreased relative to the entire calmodulin. The binding of heme-CO is specific as demonstrated by the discrimination of the calmodulin, troponin C, and parvalbumin pockets. The interaction of heme-CO with active (calcium-bound) CaM is rapid (ms) as determined by stopped flow measurements. No difference in kinetics was observed for mixing inactive (calcium free) CaM with a solution of [heme-CO plus calcium], indicating that the calcium-binding step and subsequent change in protein conformation are rapid.

Published

1993

7. Human erythrocyte band 3 polymorphism (band 3 Memphis): characterization of the structural modification (Lys 56----Glu) by protein chemistry methods.

Author

Yannoukakos D, Vasseur C, Driancourt C, Blouquit Y, Delaunay J, Wajcman H, and Bursaux E

Subjects

Anion Exchange Protein 1, Erythrocyte genetics, Anion Exchange Protein 1, Erythrocyte metabolism, Chymotrypsin metabolism, Cyanogen Bromide, Electrophoresis, Polyacrylamide Gel, Glutamates, Glutamic Acid, Heterozygote, Humans, Lysine, Peptide Fragments chemistry, Peptide Mapping, Serine Endopeptidases metabolism, Stilbenes metabolism, Trypsin metabolism, Anion Exchange Protein 1, Erythrocyte chemistry, Polymorphism, Genetic

Abstract

Band 3 variants occur rather frequently in different populations. Based on sodium dodecyl sulfate (SDS)-polyacrylamide electrophoretic properties, a widespread polymorphism (band 3 Memphis) has been previously described. It corresponds to a protein that has been hypothesized to be elongated in its N-terminal cytoplasmic domain. Band 3 from a heterozygote subject for this polymorphism and that displays a normal reactivity towards stilbene disulfonates has been isolated and its primary structure determined by protein chemistry. Reverse-phase high performance liquid chromatography tryptic peptide mapping showed, as the only difference with controls, that the enzymatic cleavage between the two N-terminal peptides did not occur, yielding a 69 residue-long fragment. Further cleavages of this peptide (cyanogen bromide, V8 protease), amino acid composition, and sequence analyses demonstrated that the lysine at position 56 was replaced by a glutamic acid. Thus, surprisingly, a single amino acid change is responsible for the large difference in the electrophoretic behavior. This result suggests that single amino acid substitutions may similarly be involved in the structural modification of several other protein variants, described as elongated or shortened based only on SDS-polyacrylamide electrophoresis studies. When deletions/insertions were confirmed by sequence analysis, their extent was often different from that expected from electrophoresis.

Published

1991

8. A new hemoglobin variant found during investigations of diabetes mellitus: Hb Pavie [alpha 135 (H18) Val----Glu].

Author

Wajcman H, Blouquit Y, Riou J, Kister J, Poyart C, Soria J, and Galacteros F

Subjects

Amino Acid Sequence, Amino Acids analysis, Chromatography, High Pressure Liquid, Hemoglobins, Abnormal metabolism, Humans, Isoelectric Focusing, Molecular Sequence Data, Diabetes Mellitus blood, Hemoglobins, Abnormal isolation & purification

Abstract

Hb Pavie [alpha 135 (H18) Val----Glu], found during HbA1c measurement in a patient of Italian origin investigated for diabetes mellitus, exemplifies how the presence of an abnormal hemoglobin interferes with the measurement of glycated hemoglobin. This variant hemoglobin migrates as Hb A1c on polyacrylamide gel isoelectric focusing (IEF) and therefore hindered the estimation of glycated hemoglobin by this method. By ion-exchange high-performance liquid chromatography (IE-HPLC) Hb Pavie was eluted as a shoulder of the major component and the corresponding glycated fraction together with Hb A1b. Hb Pavie was purified in order to determine how its functional properties may modify red cell survival. The only functional abnormality observed was a slight decrease of the oxygen affinity, and therefore the total amount of glycated hemoglobin was not expected to be decreased by a shortening of the red cell survival.

Published

1990

9. Glycosylated haemoglobin in patients on venesection therapy for haemochromatosis.

Author

Saddi R, Wajcman H, Eschwege E, Levy R, and Duchateau A

Subjects

Blood Glucose analysis, Diabetes Mellitus blood, Hemochromatosis blood, Hemoglobin A analysis, Humans, Bloodletting, Glycosides analysis, Hemochromatosis therapy, Hemoglobin A analogs & derivatives

Published

1980

10. Fast fluctuations of glycosylated hemoglobins. II. Hemoglobin A1c determination and oral glucose tolerance test.

Author

Kitzis A, Baudis M, Auge MC, Gachon AM, Dastugue B, and Wajcman H

Subjects

Diabetes Mellitus blood, Glucose Tolerance Test, Glycated Hemoglobin metabolism, Humans, Blood Glucose metabolism, Glycated Hemoglobin analysis

Published

1982

11. Quantitation of hemoglobin A1c: a rapid, automated precision-chromatography technique.

Author

Wajcman H, Dastugue B, and Labie D

Subjects

Autoanalysis, Chromatography, Diabetes Mellitus blood, Humans, Methods, Hemoglobin A analysis

Abstract

Hemoglobin A1c is increased in patients with diabetes mellitus and its level reflects the status of blood glucose equilibrium over a period of several weeks. The practical use of its estimation was hampered by technical difficulties in investigating large series of samples. In order to apply this examination for routine purposes we describe in this paper acceleration and full automatization of the original chromatographic method allowing quantitation of hemoglobin A1c in 45 min.

Published

1979

12. Isolation of human haemoglobin variants with altered Bohr effect. Application to haemoglobin Rainier.

Author

Rochette J, Baudin V, Bohn B, Poyart C, and Wajcman H

Subjects

Chromatography, High Pressure Liquid methods, Hemoglobins, Abnormal metabolism, Humans, Hydrogen-Ion Concentration, Middle Aged, Polycythemia blood, Hemoglobins, Abnormal isolation & purification, Oxyhemoglobins metabolism

Abstract

Isoelectric focusing on polyacrylamide gel in the absence of haem ligands represents a useful, convenient and rapid procedure to isolate silent Hb variants in their native forms, provided that they exhibit an abnormal Bohr effect. The amount of material which is eluted is sufficient for both a limited functional study and a structural determination using microscale high-performance liquid chromatography. This is exemplified by the isolation and the study of Hb Rainier.

Published

1986

13. [Genetic polymorphism of drepanocytosis].

Author

Pagnier J, Wajcman H, Baudin V, and Labie D

Subjects

Africa, Central, Africa, Western, Chromosome Deletion, DNA Restriction Enzymes metabolism, Fetal Hemoglobin genetics, Genetic Linkage, Globins genetics, Haploidy, Hemoglobin, Sickle genetics, Humans, Thalassemia genetics, Anemia, Sickle Cell genetics, Deoxyribonucleases, Type II Site-Specific, Polymorphism, Genetic

Abstract

The pathophysiological mechanism of sickle cell anemia has been thoroughly studied and is now well understood, in contrast to the extreme clinical heterogeneity of the disease. A possible genetic explanation for this diversity arose from the discovery of an HpaI restriction polymorphism 3' to the beta globin gene, in linkage disequilibrium with the Hb S mutation. This linkage is unequally distributed among ethnic groups in Africa and predominantly found in Central West Africa. A multipolymorphic analysis spanning 60 Kb of the beta globin gene cluster demonstrated that the sickle mutation arose at least 3 times in 3 different geographical areas (Atlantic West Africa, Central West Africa and Equatorial Central Africa) and expanded by malaria selection. Two genetic factors seem to have epistatic effects which differ when comparing the two first groups. The alpha thalassemia gene (-alpha) is distributed equally among African Black control populations (0.10). The frequency is significantly higher in the SS patients of the Benin area (Central West Africa), whereas it is unmodified in the patients of Senegal (Atlantic West Africa). Alpha thalassemia does not seem therefore to have exercised the same selective effect in this latter group. Secondly, fetal hemoglobin is quantitatively and qualitatively different in both groups. A high G gamma phenotype (greater than 60%) is found in Senegal, whereas a low G gamma phenotype is constant in Benin, without overlap between the two series. The total production of fetal hemoglobin is statistically higher, although only moderately, so in the first group.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1985

14. Immobilized pH gradients and reversed-phase high-performance liquid chromatography: a strategy for characterization of haemoglobin variants with electrophoretic mobility identical to that of Hb A. The case of Hb San Diego.

Author

Rochette J, Righetti PG, Bosisio AB, Vertongen F, Schneck G, Boissel JP, Labie D, and Wajcman H

Subjects

Amino Acids analysis, Blood Protein Electrophoresis methods, Chromatography, High Pressure Liquid methods, Humans, Hydrogen-Ion Concentration, Hemoglobin A analysis, Hemoglobins, Abnormal analysis

Abstract

The preparative aspects of immobilized pH gradients applied to abnormal haemoglobins (Hb) is described. As shown with the example of Hb San Diego, this method is successful even with as small a difference in pHi as 0.01 pH unit. For characterization of such neutral variants, reversed-phase high-performance liquid chromatography is demonstrated to be a very efficient tool.

Published

1984

15. Fast fluctuations of glycosylated hemoglobins. I. Implications for the preparation and storage of samples for hemoglobin A1c determinations.

Author

Gachon AM, Ghaddab M, Kitzis A, Wajcman H, and Dastugue B

Subjects

Carbon Monoxide, Cold Temperature, Diabetes Mellitus blood, Glycated Hemoglobin metabolism, Hemolysis, Humans, In Vitro Techniques, Time Factors, Glycated Hemoglobin analysis

Published

1982

16. Structural and functional studies of hemoglobin Barcelona (alpha 2 beta 2 94 Asp (FG1) replaced by His). Consequences of altering an important intrachain salt bridge involved in the alkaline Bohr effect.

Author

Wajcman H, Aguilar i Bascompte JL, Labie D, Poyart C, and Bohn B

Subjects

Amino Acids analysis, Humans, Hydrogen-Ion Concentration, Isoelectric Focusing, Oxyhemoglobins metabolism, Peptide Fragments, Phytic Acid pharmacology, Polycythemia blood, Protein Binding, Pyridines, Spectrophotometry, Ultraviolet, Disulfides, Hemoglobins, Abnormal

Published

1982

17. Isoelectrofocusing: a method of multiple applications for hemoglobin studies.

Author

Krishnamoorthy R, Wajcman H, and Labie D

Subjects

Fetal Hemoglobin isolation & purification, Hemoglobin, Sickle isolation & purification, Hemoglobins, Abnormal isolation & purification, Humans, Isoelectric Focusing methods, Hemoglobins isolation & purification

Abstract

A microanalytical screening of hemoglobins by isoelectric focusing on acryl-amide gel columns is described. Addition of this technique to our regular analytical procedures revealed many mutants, praticularly some neutral ones which were not resolved by other conventional procedures. Extension of this technique to a quantitative scale permitted rapid isolation of some unstable mutants in an almost pure form ready for functional studies. The natural color of the separated components is often indicative of their nature and in cases like the sulfhemoglobin, Hbs M, they are of diagnostic value. The heme-losing, abnormal, unstable mutants, on the addition of external cyanhemin, take them up and change their isoelectric pH. This is an attractive visible procedure for their diagnosis. From all these results, it appears that isoelectric focusing as a single method brings more information than the other conventional procedures and hence can be considered as a semi-routine investigation for hemoglobin studies before deciding on a much longer procedure.

Published

1976

18. Extended application of RP-HPLC for characterization of human hemoglobin variants.

Author

Baudin V and Wajcman H

Subjects

Amino Acids analysis, Chromatography, High Pressure Liquid, Humans, Mutation, Peptide Mapping, Hemoglobins, Abnormal analysis

Abstract

The different steps for the structural study of a human hemoglobin, from protein isolation to amino acid analysis, can be achieved using as the only method reversed phase high performance liquid chromatography. HPLC allows effective and rapid separations on microquantities of material. The miniaturization of the techniques led to a new approach involving successive enzymic hydrolysis of peptides.

Published

1987

19. Rapid high-performance liquid chromatographic method for the separation of the three types of gamma-chain of human fetal haemoglobin.

Author

Baudin V and Wajcman H

Subjects

Adsorption, Anemia, Sickle Cell blood, Anemia, Sickle Cell genetics, Chromatography, High Pressure Liquid methods, Fetal Hemoglobin genetics, Genes, Humans, Spectrophotometry, Ultraviolet methods, Thalassemia blood, Thalassemia genetics, Fetal Hemoglobin analysis, Globins analysis

Published

1984

20. Electrophoretic and chromatographic techniques for the differential diagnosis of a haemoglobin abnormality: Hb E heterozygosity.

Author

Bosisio AB, Rochette J, Wajcman H, Gianazza E, and Righetti PG

Subjects

Chromatography, High Pressure Liquid, Hemoglobin A2 analysis, Heterozygote, Humans, Hydrogen-Ion Concentration, Isoelectric Focusing, Thalassemia blood, Hemoglobin E genetics, Hemoglobinopathies diagnosis, Hemoglobins, Abnormal genetics

Abstract

A method is described for separating haemoglobin (Hb) E (beta 26 Gly----Lys) from Hb A2 (a normal minor Hb component in adult blood). The technique allows the distinction between subjects carrying beta-thalassaemia trait and patients who are simultaneously alpha-thalassaemic and heterozygous for Hb E, the standard electrophoretic pattern often being similar in these two circumstances. Complete separation between Hb E and Hb A2 (2 mm empty space in between) is obtained by isoelectric focusing in immobilized pH gradients in an ultra-narrow pH 7.55-7.65 gradient. The apparent pI values of the two species (at 10 degrees C and at an average ionic strength of 5.6 mequiv. l-1) have been calculated to be 7.603 for Hb E and 7.607 for Hb A2. Thus, the system reported here affords a resolution of at least 0.004 pH unit.

Published

1985

21. Separation of pure toxic peptides from a beta-gliadin subfraction using high-performance liquid chromatography.

Author

Jos J, de Tand MF, Arnaud-Battandier F, Boissel JP, Popineau Y, and Wajcman H

Subjects

Amino Acids analysis, Chemical Phenomena, Chemistry, Child, Chromatography, High Pressure Liquid methods, Culture Techniques, Humans, Hydrolysis, Intestinal Mucosa analysis, Molecular Weight, Peptide Fragments analysis, Gliadin analysis, Peptides isolation & purification, Plant Proteins analysis

Abstract

The beta v subfraction was isolated from peptic-tryptic digests of beta-gliadin by chromatography on Biogel P-10 and applied to a Lichrosorb RP-18 or a mu-Bondapak C-18 column. Fractionation was achieved using reverse-phase high-performance liquid chromatography with a linear gradient of acetonitrile in ammonium acetate. A better resolution was obtained with the mu-Bondapak column. The first-eluted peptides a, b and c1 appeared to be well purified and apparently uncontaminated. Analysis of peptides a and b showed that they contained 40 to 42% glutamine/glutamic acid, 20 to 23% proline, 14 to 16% valine and 8 to 10% leucine. They had valine as the N-terminal amino acid and their molecular mass was estimated as 5500 using sodium dodecylsulfate electrophoresis after dansylation. Peptide c1 differed from peptides a and b in containing less valine and leucine and additional amino acids such as threonine, phenylalanine and tyrosine. In addition, it had a lower molecular mass (approximately 5000) and serine as the N-terminal amino acid. Peptide b exhibited an obvious cytotoxicity for cultured coeliac jejunal mucosa at a very low concentration (0.01 g/l) and was the most toxic peptide.

Published

1983

22. Investigation of the tetramer-dimer equilibrium in haemoglobin solutions by high-performance size-exclusion chromatography on a diol column.

Author

Baudin-Chich V, Marden M, and Wajcman H

Subjects

Chromatography, Gel, Hemoglobinopathies blood, Humans, Hydrogen-Ion Concentration, Oxygen blood, Hemoglobins isolation & purification

Abstract

High-performance size-exclusion chromatography on a diol grafted column was applied to study the tetramer-dimer equilibrium in haemoglobin solution. Human haemoglobin A, isolated alpha A and beta A subunits and haemoglobin variants with structural modifications located at the interface between subunits were used as models. The elution volume of the subunits was found to deviate strongly from that expected from only a gel permeation mechanism and therefore ionic interactions are likely to participate in the protein retention. Experimental results and computer simulation indicate that the individual elution bands corresponding to the discrete components (tetramer, dimer, monomer) can be resolved under certain conditions. In general both the equilibrium and kinetic interconversion parameters must be considered. Single tetramer elution bands were observed from haemoglobin in the concentration range measurable, although the influence of dimers could be seen in the shape and shift of the profile. beta Chains showed resolved peaks for the tetramer-dimer forms.

Published

1988

23. Structure and function of haemoglobin Barcelona Asp FG1(94) beta leads to His.

Author

Phillips SE, Perutz MF, Poyart C, and Wajcman H

Subjects

Hemoglobin A, Humans, Models, Molecular, X-Ray Diffraction, Hemoglobins, Abnormal

Published

1983