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4. Direct effects of sex steroid hormones on adipose tissues and obesity.

Author

Mayes JS and Watson GH

Subjects
Adipose Tissue anatomy & histology, Animals, Female, Humans, Lipid Metabolism, Male, Mice, Rats, Sex Characteristics, Sheep, Species Specificity, Adipose Tissue metabolism, Body Composition physiology, Gonadal Steroid Hormones physiology, Obesity metabolism
Abstract

Sex steroid hormones are involved in the metabolism, accumulation and distribution of adipose tissues. It is now known that oestrogen receptor, progesterone receptor and androgen receptor exist in adipose tissues, so their actions could be direct. Sex steroid hormones carry out their function in adipose tissues by both genomic and nongenomic mechanisms. In the genomic mechanism, the sex steroid hormone binds to its receptor and the steroid-receptor complex regulates the transcription of given genes. Leptin and lipoprotein lipase are two key proteins in adipose tissues that are regulated by transcriptional control with sex steroid hormones. In the nongenomic mechanism, the sex steroid hormone binds to its receptor in the plasma membrane, and second messengers are formed. This involves both the cAMP cascade and the phosphoinositide cascade. Activation of the cAMP cascade by sex steroid hormones would activate hormone-sensitive lipase leading to lipolysis in adipose tissues. In the phosphoinositide cascade, diacylglycerol and inositol 1,4,5-trisphosphate are formed as second messengers ultimately causing the activation of protein kinase C. Their activation appears to be involved in the control of preadipocyte proliferation and differentiation. In the presence of sex steroid hormones, a normal distribution of body fat exists, but with a decrease in sex steroid hormones, as occurs with ageing or gonadectomy, there is a tendency to increase central obesity, a major risk for cardiovascular disease, type 2 diabetes and certain cancers. Because sex steroid hormones regulate the amount and distribution of adipose tissues, they or adipose tissue-specific selective receptor modulators might be used to ameliorate obesity. In fact, hormone replacement therapy in postmenopausal women and testosterone replacement therapy in older men appear to reduce the degree of central obesity. However, these therapies have numerous side effects limiting their use, and selective receptor modulators of sex steroid hormones are needed that are more specific for adipose tissues with fewer side effects.

Published
2004
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5. Melanoma vaccines as a therapeutic option.

Author

McGee JM, Price JA 3rd, Mayes JS, Patten MR, and Malnar KF

Subjects
Cause of Death, Humans, Incidence, Melanoma epidemiology, Melanoma immunology, Prognosis, Skin Neoplasms epidemiology, Skin Neoplasms immunology, Survival Analysis, Treatment Outcome, Melanoma prevention & control, Skin Neoplasms prevention & control, Vaccination methods
Abstract

Background: In 1998, 41,600 new cases of melanoma with 7,300 deaths were expected. Worldwide, the incidence has risen 5% a year against a backdrop of generally decreasing cancer trends. Later stages of melanoma carry a severe prognosis. The need for newer, more effective therapeutic strategies for cancer is obvious. For melanoma, early diagnosis and surgical treatment are the only options that are currently curative. Chemotherapy and radiation therapy are of limited efficacy., Methods: We reviewed the various forms of immunotherapy, concentrating on vaccine therapy. We then reviewed the history of our own vaccine in the context of the field of immunotherapy, and compared efficacy, immune response, production methods, and survival., Results: Survival is improved among recipients of melanoma vaccine when compared with patients receiving conventional therapy., Conclusions: Imnmunotherapy in the form of melanoma vaccines is better than conventional therapy and is trending toward purer antigenic preparations.

Published
1999
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6. Comparison of melanoma antigens in whole tumor vaccine to those from IIB-MEL-J cells.

Author

McGee JM, Patten MR, Malnar KF, Price JA 3rd, Mayes JS, and Watson GH

Subjects
Antibodies, Neoplasm immunology, Cancer Vaccines immunology, Humans, Melanoma blood, Melanoma pathology, Molecular Weight, Neoplasm Staging, Recurrence, Tumor Cells, Cultured, Antigens, Neoplasm immunology, Cancer Vaccines therapeutic use, Melanoma immunology, Melanoma therapy
Abstract

Immunotherapy for melanoma shows promise. Our previous whole tumor (WT) vaccine was noted to have positive clinical effects. We have now developed a new, safer melanoma vaccine that is derived from IIB-MEL-J tissue culture (TC) cells. In this study, we compare by Western blot analyses the antigens in the WT vaccine to antigens in the TC vaccine. Sera from 12 WT vaccine recipients, 8 melanoma patients who received no immunotherapy, and 8 controls served as a source of antibodies to investigate potential antigens in the vaccines. Three major antigenic peptides with approximate molecular weighs of 46, 40, and 36 kDA were present in both vaccines, while two other antigenic peptides with approximate molecular weighs of 68 and 48 kDA were present only in the TC vaccine. The reaction was similar between the patients who received the WT vaccine and those who did not receive the vaccine. Some of the individuals who did not have melanoma showed some reaction, but not to the extent of the melanoma patients. The intensity of immunostaining was greater for the TC vaccine when compared to the WT vaccine, indicating that these proteins are in a higher concentration in the TC vaccine. This new vaccine from IIB-MEL-J tissue culture cells provides a higher yield and a much more consistent source of potentially clinically relevant antigens without risk of infection or contamination by other irrelevant materials.

Published
1999
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7. Regional differences and up-regulation of progesterone receptors in adipose tissues from oestrogen-treated sheep.

Author

Mayes JS, McCann JP, Ownbey TC, and Watson GH

Subjects
Adipose Tissue drug effects, Animals, Blotting, Western, Centrifugation, Density Gradient, Cytosol metabolism, Female, Protein Binding, Uterus metabolism, Adipose Tissue metabolism, Estradiol pharmacology, Receptors, Progesterone metabolism, Sheep metabolism, Up-Regulation
Abstract

Differing risk factors between men and women for a number of vascular and metabolic diseases have been linked to regional obesity. The differences in the distribution of adipose tissues between men (abdominal or upper-body obesity) and women (gluteal/femoral or lower body obesity) suggest a role for sex steroids in the regional distribution of fat. Previous work from this laboratory has shown the presence of oestrogen receptor (ER) in gluteal, perirenal and omental adipose tissues of ewes with similar physical characteristics to the ER in uterine tissue. The concentration profile for adipose ER was gluteal > perirenal > omental. In this report, we determined the physiological significance of adipose ERs by showing an up-regulation of the progesterone receptor (PR) in adipose tissues after oestrogen treatment in a fashion similar to that seen in a major responsive tissue such as uterus. Using PR antibodies (PR-6 and C-262), Western blot analysis of PR from oestrogen-treated sheep indicated that PR was induced in uterus >>> gluteal adipose > perirenal adipose consistent with the concentration of ER contained in these tissues. PR could not be detected by Western blotting in omental adipose tissue from oestrogen-treated animals or in gluteal, perirenal and omental adipose tissues from untreated animals. Sucrose gradient profiles of progestin (R-5020) binding from uterus and gluteal adipose tissues of oestrogen-treated ewes showed specific binding in both the 5S and 9S regions of the gradient, while perirenal and omental adipose tissue had only the 5S peak. The amount of specific binding was increased with oestrogen treatment in all the tissues. When gluteal adipose tissue cytosol was preincubated with PR antibody (C-262) to prevent binding of ligand and subjected to sucrose gradient analysis, both the 5S and 9S regions were diminished, suggesting that both peaks contained PR. Dilution of uterine cytosol resulted in an increase in the ratio of the 5S to the 9S peak, indicating that the 9S PR complex dissociates at low concentrations; this may be the reason why only the 5S peak was observed in perirenal and omental adipose tissues. These data offer further support for a direct role of sex steroids in regional adipose accretion and metabolism.

Published
1996
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8. Intrauterine injection of ovine interferon-tau alters oestrogen receptor and oxytocin receptor expression in the endometrium of cyclic ewes.

Author

Spencer TE, Ing NH, Ott TL, Mayes JS, Becker WC, Watson GH, Mirando MA, and Brazer FW

Subjects
Analysis of Variance, Animals, Base Sequence, Cloning, Molecular, DNA Primers, DNA, Complementary, Endometrium cytology, Endometrium drug effects, Female, Immunohistochemistry, Interferon Type I administration & dosage, Interferon Type I biosynthesis, Molecular Sequence Data, Polymerase Chain Reaction, Pregnancy Proteins administration & dosage, Pregnancy Proteins biosynthesis, Progesterone blood, RNA, Messenger analysis, RNA, Messenger biosynthesis, Receptors, Oxytocin analysis, Receptors, Progesterone analysis, Receptors, Progesterone biosynthesis, Recombinant Proteins administration & dosage, Recombinant Proteins biosynthesis, Recombinant Proteins pharmacology, Reference Values, Sheep, Time Factors, Uterus, Endometrium metabolism, Estrus metabolism, Gene Expression drug effects, Interferon Type I pharmacology, Pregnancy Proteins pharmacology, Receptors, Oxytocin biosynthesis
Abstract

This study determined the effects of intrauterine injections of recombinant ovine interferon-tau; (roIFN-tau; 2 x 10(7) antiviral units/day) or control proteins (6 mg/day) from day 11 to day 14 post-oestrus = day 0) on endometrial expression of receptors fro oestrogen, progesterone and oxytocin in cyclic ewes. Plasma concentrations of progesterone were greater on day 15 in ewes receiving roIFN-tau compared with control proteins (P < 0.02, treatment x day). Ewes injected with roIFN-tau had lower endometrial levels or oestrogen receptor mRNA (P > 0.10) and protein (P < 0.01) on day 15 compared with ewes receiving control proteins. In situ hybridization analysis indicated that oestrogen receptor mRNA was more abundant in the luminal and glandular epithelium of control ewes compared with roIFN-tau-treated ewes. Immunoreactive oestrogen receptor was also present in the luminal and glandular epithelium of control, but not roIFN-tau-treated ewes. Endometrial levels of progesterone receptor mRNA and protein were not different (P > 0.10) between control and roIFN-tau-treated ewes. In situ hybridization analyses indicated that progesterone receptor mRNA abundance was low in endometrial epithelium and stroma of both control and roIFN-tau-injected ewes. Immunoreactive progesterone receptors were present in the endometrial stroma and epithelium of control ewes, but confined to the stroma of roIFN-tau-treated ewes. Oxytocin receptor density was lower (P < 0.01) in the endometrium of ewes injected with roIFN-tau than control proteins; however, oxytocin receptor affinity was not affected (P > 0.10) by treatment. Concentrations of 13,14-dihydro-15-ketoprostaglandin F2a (PGFM) were not increased by exogenous oxytocin administration in control and roIFN-tau-treated ewes on days 10 or 12 post-oestrus. However, on day 14, control ewes responded to oxytocin with increased plasma concentrations of PGFM, whereas ewes receiving roIFN-tau remained unresponsive to oxytocin. These results indicate that the an tiluteolytic effects of IFN-tau are to prevent increases in endometrial oestrogen receptor MRNA and protein and oxytocin receptor density which abrogates uterine release of prostaglandin F2a during maternal recognition of pregnancy. IFN-tau may inhibit the synthesis of oestrogen receptor mRNA by a transcriptional or post-transcriptional regulatory mechanism to suppress oxytocin receptor formation during early pregnancy in ewes.

Published
1995
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9. Biochemical and immunological characterization of oestrogen receptor in the cytosolic fraction of gluteal, omental and perirenal adipose tissues from sheep.

Author

Watson GH, Manes JL, Mayes JS, and McCann JP

Subjects
Adrenalectomy, Animals, Binding, Competitive, Blotting, Western, Buttocks, Centrifugation, Density Gradient, Female, Kidney, Omentum, Ovariectomy, Radioligand Assay, Sheep, Uterus chemistry, Adipose Tissue chemistry, Cytosol chemistry, Receptors, Estrogen analysis
Abstract

Determination of the presence and characterization of oestrogen receptors (ERs) in subcutaneous and internal fat depots were performed and compared with ERs in the uterus using ligand binding and immunological techniques. Successful and consistent measurement of ERs in ovine adipose tissue could only be accomplished in animals depleted of endogenous sex steroids by combined ovariectomy and adrenalectomy. Scatchard, sucrose gradient and Western blot analyses all confirmed the presence of ERs in the cytosolic fractions of various adipose and uterine tissues from ovariectomized-adrenalectomized ewes. The approximate Kd values of 0.1-0.4 nmol/l for oestradiol binding in cytosolic fractions of gluteal, omental and perirenal adipose tissues were similar to the expected high affinity binding of Kd 0.35 nmol/l observed in uterine tissue. The binding was specific for oestrogens, as unlabelled diethylstilboestrol and oestradiol effectively competed with labelled hormone for receptor sites and progesterone, R5020, testosterone and dexamethasone all failed to compete. Mean (+/- S.E.M.) concentrations of ERs, expressed as fmol specific binding sites per mg protein, were much lower (P < 0.05) in adipose tissues than in uterine tissue (975 +/- 33). However, the content of ERs was greater (P < 0.05) in subcutaneous gluteal fat (11.5 +/- 0.8) than in the internal omental or perirenal fat (5 +/- 0.6) depots. ERs from adipose and uterine tissues both migrated as moieties of 8S on 5-20% sucrose gradients. Western blot analysis of ERs from uterine and adipose tissues in the presence of protease inhibitors demonstrated an immunostaining band with a molecular mass of 67 kDa.(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1993
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10. alpha-galactosidase A from human placenta. Stability and subunit size.

Author

Mayes JS and Beutler E

Subjects
Electrophoresis, Disc, Epitopes, Female, Hot Temperature, Humans, Hydrogen-Ion Concentration, Molecular Weight, Pregnancy, Protein Denaturation, alpha-Galactosidase immunology, Galactosidases isolation & purification, Placenta enzymology, alpha-Galactosidase isolation & purification
Abstract

alpha-Galactosidase A (alpha-D-galactoside galactohydrolase, EC 3.2.1.22) was purified from human placenta. The purified enzyme showed one major band on polyacrylamide gel electrophoresis and a single precipitin line on double immunodiffusion. Electrophoresis of the purified, S-carboxymethylated enzyme on sodium dodecyl sulfate polyacrylamide gel showed one component with a molecular weight of about 65 000, but electrophoresis of the non-S-carboxymethylated enzyme showed two components, a major band with a molecular weight of 67 500 and a diffuse band with a molecular weight of 47 000. We suggest that the smaller diffuse component is a degradation product and that the enzyme is a dimer with a molecular weight of approximately 150 000 and a subunit of molecular weight of about 67 500. Antibody raised against the purified enzyme quantitatively precipitated alpha-galactosidase A, but not alpha-galactosidase in Fabry's disease fibroblasts. The alpha-galactosidase A is very heat labile and pH sensitive. It is most stable in concentrated solution at low temperature and at a pH of 5.0 to 6.0. When added to plasma at 37 degrees C, it has a half-life of only 17 min. This imposes a serious obstacle to its use in the treatment of Fabry's disease.

Published
1977
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11. Activator protein required for the enzymatic hydrolysis of cerebroside sulfate. Deficiency in urine of patients affected with cerebroside sulfatase activator deficiency and identity with activators for the enzymatic hydrolysis of GM1 ganglioside and globotriaosylceramide.

Author

Li SC, Kihara H, Serizawa S, Li YT, Fluharty AL, Mayes JS, and Shapiro LJ

Subjects
Animals, Enzyme Activation, G(M2) Ganglioside metabolism, Glycosphingolipids urine, Hexosaminidases metabolism, Humans, Hydrolysis, Immunodiffusion, Immunosorbent Techniques, Proteinuria, Rats, Saposins, alpha-Galactosidase metabolism, beta-Galactosidase metabolism, beta-N-Acetylhexosaminidases, G(M1) Ganglioside metabolism, Gangliosides metabolism, Globosides metabolism, Glycosphingolipids metabolism, Protein Deficiency, Proteins, Trihexosylceramides
Abstract

Urine specimens from two sibs affected with cerebroside sulfatase activator deficiency were examined to ascertain whether the deficiency of the supplementary activator protein required for the enzymatic hydrolysis of cerebroside sulfate was also evident in urine. Material from chromatographic fractionations was examined for the activator activity to avoid ambiguities resulting from protein inhibition. There were substantial deficits in all chromatographic fractions corresponding to activator-containing fractions of control urines. Since patient urines contained elevated amounts of lactosylceramide, digalactosylceramide, and globotriaosylceramide and since similarities between activators for cerebroside sulfate and GM1 ganglioside hydrolyses had been noted previously, the chromatographic fractions were also examined for activators in other glycosphingolipid hydrolase systems. There was coincidence of activators for the GM1 ganglioside/beta-galactosidase and the globotriaosylceramide/alpha-galactosidase A reactions with the cerebroside sulfatase activator in control urine fractions, and the patients' urines were deficient in activator activities for the three reactions. Identity of the three activators was suggested and antiserum to purified GM1 ganglioside activator was used to test this possibility. There were depressed levels of cross-reacting material in fractions of patient urines by Ouchterlony double diffusion and in unfractionated urine by enzyme-linked immunosorbent assay. Purified activators for the cerebroside sulfate and GM1 ganglioside systems showed lines of identity with no spurring on Ouchterlony double diffusion, identical mobility on immunoelectrophoresis, and similar stimulatory activities toward hydrolysis of the three glycosphingolipid species by their respective enzymes. Finally, the three activator activities were retained by anti-GM1-activator IgG coupled to Sepharose 4B. The results suggest strongly that the same protein entity serves as activator for the enzymatic hydrolysis of cerebroside sulfate, GM1 ganglioside, and globotriaosylceramide.

Published
1985

12. Loss of electron-dense lamellar material from Fabry's disease fibroblasts after enzyme replacement.

Author

Sifers RN, Mayes JS, and Nordquist RE

Subjects
Adult, Cells, Cultured, Culture Media, Fabry Disease enzymology, Fibroblasts ultrastructure, Humans, Male, Microscopy, Electron, Fabry Disease ultrastructure, Galactosidases metabolism, alpha-Galactosidase metabolism
Abstract

Cultured fibroblasts from a patient with Fabry's disease were treated with alpha-galactosidase A. The cells internalized the enzyme via a receptor-mediated transport system, resulting in the uptake of enzyme to 50% of the activity of normal cells. Following uptake of the enzyme and incubation for 9 days, a loss of electron-dense lamellar material within membrane-bound residual bodies was detected by electron microscopy. Morphometric analysis of electron micrographs showed that the percentage volume of cytoplasm occupied by electron-dense lamellar material in Fabry's disease fibroblasts decreased to near normal after treatment with enzyme. These results indicate that the ultrastructural abnormalities of Fabry's disease cells can be corrected by enzyme replacement, at least in cultured fibroblasts.

Published
1983
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13. Endocytosis of lysosomal alpha-galactosidase A by cultured fibroblasts from patients with Fabry disease.

Author

Mayes JS, Cray EL, Dell VA, Scheerer JB, and Sifers RN

Subjects
Adult, Cells, Cultured, Endocytosis, Fabry Disease pathology, Fibroblasts metabolism, Half-Life, Humans, In Vitro Techniques, Lysosomes enzymology, Male, Fabry Disease enzymology, Galactosidases metabolism, alpha-Galactosidase metabolism
Abstract

The endocytosis of alpha-galactosidase A was studied in cultured fibroblasts from patients with Fabry disease. Alpha-galactosidase A was purified from human placenta by chromatography on concanavalin A-Sepharose, DEAE-cellulose, and N-epsilon-aminocaproyl-alpha-D-galactosylamine-Sepharose. Separation of the high-uptake form of the enzyme from the low-uptake form was accomplished by chromatography on ECTEOLA-cellulose. With the high-uptake form of the enzyme, the uptake was linear at low concentrations of enzyme and had a Kuptake of 0.01 U/ml of medium that corresponds to a Km of 5.0 x 10(-9) M. At high concentrations of enzyme, it became saturated. The high-uptake form could be converted to the low-uptake form by treatment with acid phosphatase. Mannose-6-P strongly inhibited the active uptake of the enzyme. Once taken up into the lysosomes of Fabry disease fibroblasts, alpha-galactosidase A activity was rapidly lost in the first 2 days of incubation at 37 degrees C, but was fairly stable for the next 6 days. The half-life of internalized alpha-galactosidase A activity was calculated to be 4 days. Crosslinking of the enzyme with hexamethylene diisocyanate did not increase the intracellular stability of alpha-galactosidase A activity.

Published
1982

14. Partial deletion 21: case report with biochemical studies and review.

Author

Carpenter NJ, Mayes JS, Say B, and Wilson DP

Subjects
Abnormalities, Multiple genetics, Child, Preschool, Chromosome Mapping, Cystathionine beta-Synthase metabolism, Female, Humans, Superoxide Dismutase metabolism, Chromosome Deletion, Chromosomes, Human, Pair 21, Chromosomes, Human, Pair 4, Intellectual Disability genetics, Translocation, Genetic
Abstract

An unbalanced translocation of a portion of the long arm of chromosome 21 to the short arm of chromosome 4 resulted in a partial deletion of chromosome 21 (pter----q21.05) and in the loss of the telomere of 4p. The phenotype of the child included asymmetrical facies, microcephaly, short stature, hypotonia, and psychomotor retardation associated with frequent infections. Normal SOD-1 activity in red blood cells and fibroblasts and normal cystathionine beta synthase activity in fibroblasts suggest that these gene loci are distal to 21q21.05.

Published
1987
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15. Purification, properties, and isozyme pattern of galactose-1-phosphate uridyl transferase from calf liver.

Author

Mayes JS

Subjects
Animals, Calcium pharmacology, Cattle, Magnesium pharmacology, Manganese pharmacology, Molecular Weight, Potassium Chloride pharmacology, Sodium Chloride pharmacology, UTP-Hexose-1-Phosphate Uridylyltransferase metabolism, Liver enzymology, Nucleotidyltransferases isolation & purification, UTP-Hexose-1-Phosphate Uridylyltransferase isolation & purification
Published
1976
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16. Differential assay for lysosomal alpha-galactosidases in human tissues and its application to Fabry's disease.

Author

Mayes JS, Scheerer JB, Sifers RN, and Donaldson ML

Subjects
Acetylgalactosamine pharmacology, Adult, Cells, Cultured, Fabry Disease genetics, Female, Fibroblasts enzymology, Galactosides, Genetic Carrier Screening, Hexosaminidases antagonists & inhibitors, Humans, Hymecromone analogs & derivatives, Lysosomes enzymology, Male, alpha-N-Acetylgalactosaminidase, Fabry Disease enzymology, Galactosidases metabolism, Hexosaminidases metabolism, alpha-Galactosidase metabolism
Abstract

A simple and sensitive fluorometric method has been described for the differential determination of the activity of lysosomal alpha-galactosidase A and alpha-galactosidase B. The procedure employs 4-methylumbelliferyl-alpha-D-galactopyranoside as substrate and N-acetylgalactosamine as an inhibitor of alpha-galactosidase B, but not of alpha-galactosidase A to differentiate the two activities. This method was shown to be applicable in the differentiation of the two enzyme activities in human tissues and in the diagnosis of the heterozygous and hemizygous genotypes for Fabry's disease in cultured skin fibroblasts.

Published
1981
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17. Plasma and submandibular saliva lysosomal enzymes in cystic fibrosis.

Author

Oglesbee LH, Seale TW, Mayes JS, Flux M, Young SK, and Renner OM

Subjects
Acid Phosphatase blood, Adolescent, Adult, Child, Child, Preschool, Drug Stability, Female, Galactosidases metabolism, Hot Temperature, Humans, Lysosomes enzymology, Male, Mannosidases blood, alpha-Glucosidases metabolism, alpha-L-Fucosidase metabolism, alpha-Mannosidase, Acid Phosphatase metabolism, Cystic Fibrosis enzymology, Mannosidases metabolism, Saliva enzymology, Submandibular Gland enzymology
Abstract

This study determined in a blind fashion the activity levels and thermostability properties of two lysosomal hydrolytic enzymes, acid phosphatase and alpha-mannosidase, in plasma samples from 25 cystic fibrosis (CF) patients and 25 age- and sex-matched normal controls. Mean alpha-mannosidase activity (3.2 +/- 1.0 mU/ml) and acid phosphatase activities (6.5 +/- 2.9 mU/ml) in CF patients were not significantly different from those found in normal individuals (2.8 +/- 0.7 and 7.6 +/- 3.4 mU/ml, respectively). Using stringent conditions no differences in thermostability properties of these enzymes were found between plasma from CF patients as compared to that of normal controls. When activity levels of these enzymes and of four additional hydrolytic enzymes, alpha-L-fucosidase, alpha-galactosidase, alpha-glucosidase and beta-galactosidase, were determined in submandibular saliva, no significant differences in enzyme levels between CF and age- and sex-matched controls were noted nor were thermostability differences found. Our data do not support the concept that altered properties of these enzymes are useful as markers for detection of CF homozygotes and heterozygotes, nor the hypothesis that the defect underlying this disease is a deficiency of post-translational modification of glycoproteins leading to their mis-compartmentalization and qualitative alteration.

Published
1984
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19. The relationship of galactose-1-phosphate accumulation and uridyl transferase activity to the differential galactose toxicity in male and female chicks.

Author

Mayes JS, Miller LR, and Myers FK

Subjects
Animals, Brain metabolism, Chickens, Dietary Carbohydrates, Female, Galactosemias metabolism, Isomerases metabolism, Liver metabolism, Male, Phosphotransferases metabolism, Sex Factors, Uracil Nucleotides, Galactose toxicity, Hexosephosphates metabolism, Nucleotidyltransferases
Published
1970
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20. The metabolism of galactose by galactosemic fibroblasts in vitro.

Author

Mayes JS and Miller LR

Subjects
Biological Transport, Carbon Radioisotopes, Cell Line, Chromatography, Paper, Fibroblasts metabolism, Galactosemias pathology, Glucose metabolism, Heterozygote, Hexosephosphates metabolism, Humans, Isotope Labeling, Time Factors, Galactose metabolism, Galactosemias metabolism, Skin metabolism
Published
1973
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21. Detection of heterozygotes for galactokinase deficiency in a human population.

Author

Mayes JS and Guthrie R

Subjects
Adult, Carbohydrate Metabolism, Inborn Errors genetics, Carbon Isotopes, Child, Child, Preschool, Culture Techniques, Erythrocytes enzymology, Female, Fibroblasts enzymology, Freezing, Humans, Hydrogen-Ion Concentration, Male, Methods, Pedigree, Time Factors, Carbohydrate Metabolism, Inborn Errors diagnosis, Galactose, Heterozygote, Phosphotransferases blood
Published
1968
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25. Galactose toxicity and activities of the galactose-metabolizing enzymes during development of the chick.

Author

Parkhurst GW and Mayes JS

Subjects
Aging, Animals, Chick Embryo, Dietary Carbohydrates, Female, Liver embryology, Liver growth & development, Male, Nucleoside Diphosphate Sugars, Sex Factors, Uracil Nucleotides, Chickens, Galactose toxicity, Isomerases metabolism, Liver enzymology, Nucleotidyltransferases metabolism, Phosphotransferases metabolism
Published
1972
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