Your search keyword '"Foecking MF"' showing total 56 results

1. Complete Genome Sequence of Kocuria palustris MU14/1.

Author

Calcutt MJ and Foecking MF

Abstract

Presented here is the first completely assembled genome sequence of Kocuria palustris, an actinobacterial species with broad ecological distribution. The single, circular chromosome of K. palustris MU14/1 comprises 2,854,447 bp, has a G+C content of 70.5%, and contains a deduced gene set of 2,521 coding sequences., (Copyright © 2015 Calcutt and Foecking.)

Published

2015

2. An Excision-Competent and Exogenous Mosaic Transposon Harbors the tetM Gene in Multiple Mycoplasma hominis Lineages.

Author

Calcutt MJ and Foecking MF

Subjects

DNA Transposable Elements genetics, Mycoplasma hominis genetics

Published

2015

3. Genome Sequence Analysis of Mycoplasma sp. HU2014, Isolated from Tissue Culture.

Author

Calcutt MJ, Szikriszt B, Póti Á, Molnár J, Gervai JZ, Tusnády GE, Foecking MF, and Szüts D

Abstract

The draft genome sequence of a novel Mycoplasma strain, designated Mycoplasma sp. HU2014, has been determined. The genome comprises 1,084,927 nucleotides and was obtained from a mycoplasma-infected culture of chicken DT40 cells. Phylogenetic analysis places this taxon in a group comprising the closely related species Mycoplasma yeatsii and Mycoplasma cottewii., (Copyright © 2015 Calcutt et al.)

Published

2015

4. Comparative analysis of the Mycoplasma capricolum subsp. capricolum GM508D genome reveals subrogation of phase-variable contingency genes and a novel integrated genetic element.

Author

Calcutt MJ and Foecking MF

Subjects

Molecular Sequence Data, Sequence Analysis, DNA, Antigenic Variation, Gene Order, Genes, Bacterial, Genetic Variation, Genome, Bacterial, Interspersed Repetitive Sequences, Mycoplasma capricolum genetics

Abstract

Mycoplasma capricolum subspecies capricolum is both a pathogen of small ruminants and a model recipient organism for gene transplantation and synthetic biology. With the availability of the complete genome of the type strain California kid (released in 2005), a draft genome of strain GM508D was determined to investigate genomic variation in this subspecies. Differences in mobile genetic element location and complement, catabolic pathway genes, contingency loci, surface antigen genes and type II restriction-modification systems highlight the plasticity and diversity within this taxon., (© FEMS 2015. All rights reserved. For permissions, please e-mail: journals.permissions@oup.com.)

Published

2015

5. Complete Genome Sequence of Mycoplasma hominis Strain Sprott (ATCC 33131), Isolated from a Patient with Nongonococcal Urethritis.

Author

Calcutt MJ and Foecking MF

Abstract

Presented here is the complete and annotated genome sequence of Mycoplasma hominis Sprott (ATCC 33131). The chromosome comprises 695,214 bp, which is approximately 30 kb larger than the syntenic genome of M. hominis PG21(T). Tetracycline resistance of strain Sprott is most probably conferred by the tetM determinant, harbored on a mosaic transposon-like structure., (Copyright © 2015 Calcutt and Foecking.)

Published

2015

6. Complete Genome Sequence of Mycoplasma yeatsii Strain GM274B (ATCC 43094).

Author

Calcutt MJ, Kent BN, and Foecking MF

Abstract

Mycoplasma yeatsii is a goat mycoplasma species that, although an obligate parasite, accommodates this lifestyle as an inapparent commensalist. High-frequency transformation has also been reported for this species. The complete 895,051-bp genome sequence of strain GM274B has been determined, enabling an analysis of the features of this potential cloning host., (Copyright © 2015 Calcutt et al.)

Published

2015

7. Complete Genome Sequence of Mycoplasma flocculare Strain Ms42T (ATCC 27399T).

Author

Calcutt MJ, Foecking MF, Heidari MB, and McIntosh MA

Abstract

Mycoplasma flocculare is a commensal or low-virulence pathogen of swine. The complete 778,866-bp genome sequence of M. flocculare strain Ms42(T) has been determined, enabling further comparison to genomes of the closely related pathogen Mycoplasma hyopneumoniae. The absence of the p97 and glpD genes may contribute to the attenuated virulence of M. flocculare., (Copyright © 2015 Calcutt et al.)

Published

2015

8. Analysis of the Complete Mycoplasma hominis LBD-4 Genome Sequence Reveals Strain-Variable Prophage Insertion and Distinctive Repeat-Containing Surface Protein Arrangements.

Author

Calcutt MJ and Foecking MF

Abstract

The complete genome sequence of Mycoplasma hominis LBD-4 has been determined and the gene content ascribed. The 715,165-bp chromosome contains 620 genes, including 14 carried by a strain-variable prophage genome related to Mycoplasma fermentans MFV-1 and Mycoplasma arthritidis MAV-1. Comparative analysis with the genome of M. hominis PG21(T) reveals distinctive arrangements of repeat-containing surface proteins., (Copyright © 2015 Calcutt and Foecking.)

Published

2015

9. Sequence Analysis of Staphylococcus hyicus ATCC 11249T, an Etiological Agent of Exudative Epidermitis in Swine, Reveals a Type VII Secretion System Locus and a Novel 116-Kilobase Genomic Island Harboring Toxin-Encoding Genes.

Author

Calcutt MJ, Foecking MF, Hsieh HY, Adkins PR, Stewart GC, and Middleton JR

Abstract

Staphylococcus hyicus is the primary etiological agent of exudative epidermitis in swine. Analysis of the complete genome sequence of the type strain revealed a locus encoding a type VII secretion system and a large chromosomal island harboring the genes encoding exfoliative toxin ExhA and an EDIN toxin homolog., (Copyright © 2015 Calcutt et al.)

Published

2015

10. Genome Sequence of Actinobacillus suis Type Strain ATCC 33415T.

Author

Calcutt MJ, Foecking MF, Mhlanga-Mutangadura T, and Reilly TJ

Abstract

The assembled and annotated genome of Actinobacillus suis ATCC 33415(T) is reported here. The 2,501,598-bp genome encodes 2,246 open reading frames (ORFs) with strain variable incursion of an integrative conjugative element into a tRNA locus. Comparative analysis of the deduced gene set should inform our understanding of pathogenesis, genomic plasticity, and serotype variation., (Copyright © 2014 Calcutt et al.)

Published

2014

11. Draft Genome Sequence of Bovine Mastitis Isolate Staphylococcus agnetis CBMRN 20813338.

Author

Calcutt MJ, Foecking MF, Fry PR, Hsieh HY, Perry J, Stewart GC, Scholl DT, Messier S, and Middleton JR

Abstract

Presented here is a draft genome sequence for Staphylococcus agnetis CBMRN 20813338, isolated from a lactating dairy cow with subclinical mastitis. The genome is approximately 2,416 kb and has 35.79% G+C content. Analysis of the deduced open reading frame (ORF) set identified candidate virulence attributes in addition to potential molecular targets for species identification., (Copyright © 2014 Calcutt et al.)

Published

2014

12. Draft Genome Sequence of Staphylococcus chromogenes Strain MU 970, Isolated from a Case of Chronic Bovine Mastitis.

Author

Fry PR, Calcutt MJ, Foecking MF, Hsieh HY, Suntrup DG, Perry J, Stewart GC, and Middleton JR

Abstract

Coagulase-negative staphylococcal species are a common cause of subclinical bovine mastitis, with Staphylococcus chromogenes being one of the most frequently identified species in these cases. The draft genome sequence of an S. chromogenes isolate (MU 970) recovered from the milk of a cow with a chronic intramammary infection is reported here., (Copyright © 2014 Fry et al.)

Published

2014

13. Complete Genome Sequence of the Bovine Mastitis Pathogen Mycoplasma californicum Strain ST-6T (ATCC 33461T).

Author

Calcutt MJ, Foecking MF, and Fox LK

Abstract

Mycoplasma californicum is one of several mycoplasmal species associated with bovine mastitis. The complete genome sequence of 793,841 bp has been determined and annotated for the M. californicum ST-6 type strain, providing a resource for the identification of surface antigens and putative pathoadaptive features., (Copyright © 2014 Calcutt et al.)

Published

2014

14. Draft Genome Sequence of Moraxella bovoculi Strain 237T (ATCC BAA-1259T) Isolated from a Calf with Infectious Bovine Keratoconjunctivitis.

Author

Calcutt MJ, Foecking MF, Martin NT, Mhlanga-Mutangadura T, and Reilly TJ

Abstract

Moraxella bovoculi is a recently identified species, recovered from the bovine eye, which is under investigation as an etiological agent of infectious bovine keratoconjunctivitis. A draft genome sequence of the Moraxella bovoculi type strain 237(T) has been determined to identify features that may be important during host colonization., (Copyright © 2014 Calcutt et al.)

Published

2014

15. Draft Genome Sequence of Fusobacterium necrophorum subsp. funduliforme Bovine Liver Abscess Isolate B35.

Author

Calcutt MJ, Foecking MF, Nagaraja TG, and Stewart GC

Abstract

Fusobacterium necrophorum is a Gram-negative anaerobic bacterium that causes foot rot and liver abscesses in cattle. F. necrophorum subsp. necrophorum and the less virulent organism F. necrophorum subsp. funduliforme are recognized. We present here a draft genome sequence of the bovine liver abscess isolate F. necrophorum subsp. funduliforme strain B35, which affords a genomic perspective of virulence and bovine adaptation.

Published

2014

16. Complete Genome Sequence of Mycoplasma bovoculi Strain M165/69T (ATCC 29104).

Author

Calcutt MJ and Foecking MF

Abstract

Bovine ocular infections compromise animal health and result in significant economic losses. Mycoplasma bovoculi is an etiological agent of conjunctivitis. Presented here is the 760,240-bp complete genome sequence of the M. bovoculi type strain M165/69(T). An analysis of the deduced proteome provides insights into the adherence and antigenic variation mechanisms of the strain.

Published

2014

17. Draft Genome Sequence of Staphylococcus simulans UMC-CNS-990, Isolated from a Case of Chronic Bovine Mastitis.

Author

Calcutt MJ, Foecking MF, Hsieh HY, Perry J, Stewart GC, and Middleton JR

Abstract

Coagulase-negative staphylococci are frequently isolated from cases of subclinical bovine mastitis. Reported here is a draft genome sequence of Staphylococcus simulans UMC-CNS-990, an isolate recovered from a chronic intramammary infection of a Holstein cow. Unexpectedly, a cluster of genes encoding gas vesicle proteins was found within the 2,755-kb genome.

Published

2013

18. Genome Sequence Analysis of Staphylococcus equorum Bovine Mastitis Isolate UMC-CNS-924.

Author

Calcutt MJ, Foecking MF, Hsieh HY, Perry J, Stewart GC, and Middleton JR

Abstract

Intramammary infections in dairy cattle are frequently caused by staphylococci, resulting in mastitis and associated economic losses. A draft genome sequence was determined for Staphylococcus equorum UMC-CNS-924, isolated from the milk of a Holstein cow, to better understand the genetic basis of its pathogenesis and adaptation to the bovine mammary gland.

Published

2013

19. Development of a novel plasmid as a shuttle vector for heterologous gene expression in Mycoplasma yeatsii.

Author

Kent BN, Foecking MF, and Calcutt MJ

Subjects

Electroporation, Escherichia coli genetics, Plasmids, Transfection, Transformation, Genetic, Gene Expression, Genetic Vectors, Genetics, Microbial methods, Molecular Biology methods, Mycoplasma genetics

Abstract

A circular plasmid, pMyBK1, was detected in Mycoplasma yeatsii strain GIH(T). Analysis of the sequence of the 3432-bp replicon identified two predicted open reading frames (ORFs), one with sequence similarity to multiple plasmid mobilization proteins and one that matches only to hypothetical ORFs encoded by integrated chromosomal elements in the sequenced genomes of two Mycoplasma species. Shuttle vectors were constructed in Escherichia coli which could be introduced into M. yeatsii at high efficiency (10(4)-10(5) per μg DNA) by electroporation. Independent deletion analysis of the two ORFs disclosed that whereas mob was dispensable, orf2 was necessary for plasmid replication or maintenance. The absence of plasmid-encoded database matches for ORF2 indicates that pMyBK1 represents a novel plasmid family. One shuttle vector was used to demonstrate heterologous expression of the Mycoplasma fermentans malp gene and was stable during multiple passages. The host-plasmid system described has potential application for genetic manipulation in a genus for which few replicative vectors are available., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published

2012

20. Complete genome sequences of Mycoplasma leachii strain PG50T and the pathogenic Mycoplasma mycoides subsp. mycoides small colony biotype strain Gladysdale.

Author

Wise KS, Calcutt MJ, Foecking MF, Madupu R, DeBoy RT, Röske K, Hvinden ML, Martin TR, Durkin AS, Glass JI, and Methé BA

Subjects

Animals, Cattle, Cattle Diseases microbiology, Molecular Sequence Data, Mycoplasma mycoides isolation & purification, Pleuropneumonia, Contagious microbiology, DNA, Bacterial chemistry, DNA, Bacterial genetics, Genome, Bacterial, Mycoplasma mycoides genetics, Sequence Analysis, DNA

Abstract

Mycoplasma mycoides subsp. mycoides small colony biotype (SC) is the high-consequence animal pathogen causing contagious bovine pleuropneumonia. We report the complete genome sequences of the pathogenic strain M. mycoides subsp. mycoides SC Gladysdale and a close phylogenetic relative, Mycoplasma leachii PG50(T), another bovine pathogen of the M. mycoides phylogenetic clade.

Published

2012

21. Genome sequence of Mycoplasma hyorhinis strain GDL-1.

Author

Calcutt MJ, Foecking MF, Rosales RS, Ellis RJ, and Nicholas RA

Subjects

Animals, Base Sequence, Molecular Sequence Data, Mycoplasma Infections microbiology, Phylogeny, Swine, Genome, Bacterial, Mycoplasma Infections veterinary, Mycoplasma hyorhinis genetics, Swine Diseases microbiology

Abstract

Mycoplasma hyorhinis impacts swine health and production in many countries, either as a primary pathogen or as a component of a polymicrobial infection. Isolates of this species are also common contaminants of tissue culture lines. The genome sequence of the cell culture isolate M. hyorhinis GDL-1 is presented herein.

Published

2012

22. Genome sequence of Mycoplasma putrefaciens type strain KS1.

Author

Calcutt MJ and Foecking MF

Subjects

Animals, Goat Diseases microbiology, Goats, Molecular Sequence Data, Mycoplasma isolation & purification, Sequence Analysis, DNA, DNA, Bacterial chemistry, DNA, Bacterial genetics, Genome, Bacterial, Mycoplasma genetics

Abstract

Mycoplasma putrefaciens is a causative agent of contagious agalactia in goats. Reported herein is the complete genome sequence of the M. putrefaciens type strain KS1.

Published

2011

23. Complete genome sequence of Mycoplasma bovis type strain PG45 (ATCC 25523).

Author

Wise KS, Calcutt MJ, Foecking MF, Röske K, Madupu R, and Methé BA

Subjects

Animals, Cattle, Genome, Bacterial, Molecular Sequence Data, Sequence Analysis, DNA, Species Specificity, Mycoplasma bovis genetics

Abstract

This complete and fully assembled genome sequence of Mycoplasma bovis type strain PG45 is the first available for this species and offers a framework for comparison with additional pathogenic isolates. The single circular chromosome of 1,003,404 bp reveals multiple gene sets and mechanisms involved in variable expression of surface antigens and the incursion of numerous and assorted mobile elements, despite its reduced size.

Published

2011

24. A versatile palindromic amphipathic repeat coding sequence horizontally distributed among diverse bacterial and eucaryotic microbes.

Author

Röske K, Foecking MF, Yooseph S, Glass JI, Calcutt MJ, and Wise KS

Subjects

Amino Acid Motifs, Amino Acid Sequence, Animals, Bacterial Proteins chemistry, Base Sequence, Genome, Bacterial genetics, Membrane Proteins chemistry, Membrane Proteins genetics, Metagenome genetics, Molecular Sequence Data, Parasites genetics, Phenotype, Phylogeny, Protein Structure, Tertiary, Tandem Repeat Sequences genetics, Bacteria genetics, Bacterial Proteins genetics, Eukaryota genetics, Gene Transfer, Horizontal, Inverted Repeat Sequences genetics, Open Reading Frames genetics

Abstract

Background: Intragenic tandem repeats occur throughout all domains of life and impart functional and structural variability to diverse translation products. Repeat proteins confer distinctive surface phenotypes to many unicellular organisms, including those with minimal genomes such as the wall-less bacterial monoderms, Mollicutes. One such repeat pattern in this clade is distributed in a manner suggesting its exchange by horizontal gene transfer (HGT). Expanding genome sequence databases reveal the pattern in a widening range of bacteria, and recently among eucaryotic microbes. We examined the genomic flux and consequences of the motif by determining its distribution, predicted structural features and association with membrane-targeted proteins., Results: Using a refined hidden Markov model, we document a 25-residue protein sequence motif tandemly arrayed in variable-number repeats in ORFs lacking assigned functions. It appears sporadically in unicellular microbes from disparate bacterial and eucaryotic clades, representing diverse lifestyles and ecological niches that include host parasitic, marine and extreme environments. Tracts of the repeats predict a malleable configuration of recurring domains, with conserved hydrophobic residues forming an amphipathic secondary structure in which hydrophilic residues endow extensive sequence variation. Many ORFs with these domains also have membrane-targeting sequences that predict assorted topologies; others may comprise reservoirs of sequence variants. We demonstrate expressed variants among surface lipoproteins that distinguish closely related animal pathogens belonging to a subgroup of the Mollicutes. DNA sequences encoding the tandem domains display dyad symmetry. Moreover, in some taxa the domains occur in ORFs selectively associated with mobile elements. These features, a punctate phylogenetic distribution, and different patterns of dispersal in genomes of related taxa, suggest that the repeat may be disseminated by HGT and intra-genomic shuffling., Conclusions: We describe novel features of PARCELs (Palindromic Amphipathic Repeat Coding ELements), a set of widely distributed repeat protein domains and coding sequences that were likely acquired through HGT by diverse unicellular microbes, further mobilized and diversified within genomes, and co-opted for expression in the membrane proteome of some taxa. Disseminated by multiple gene-centric vehicles, ORFs harboring these elements enhance accessory gene pools as part of the "mobilome" connecting genomes of various clades, in taxa sharing common niches.

Published

2010

25. Distinctive repertoire of contingency genes conferring mutation- based phase variation and combinatorial expression of surface lipoproteins in Mycoplasma capricolum subsp. capricolum of the Mycoplasma mycoides phylogenetic cluster.

Author

Wise KS, Foecking MF, Röske K, Lee YJ, Lee YM, Madan A, and Calcutt MJ

Subjects

5' Flanking Region, Amino Acid Sequence, Bacterial Proteins metabolism, Base Sequence, Genes, Bacterial, Membrane Proteins metabolism, Molecular Sequence Data, Mutation, Mycoplasma capricolum metabolism, Mycoplasma mycoides metabolism, Phylogeny, Terminal Repeat Sequences, Bacterial Proteins genetics, Genetic Variation, Membrane Proteins genetics, Mycoplasma capricolum genetics, Mycoplasma mycoides genetics

Abstract

The generation of surface variation among many divergent species of Mollicutes (mycoplasmas) occurs through stochastic expression patterns of diverse lipoprotein genes. The size and wide distribution of such variable gene sets in minimal (approximately 0.6- to 1.4-Mb) mycoplasmal genomes suggest their key role in the adaptation and survival of these wall-less monoderms. Diversity through variable genes is less clearly established among phylogenetically similar mycoplasmas, such as the Mycoplasma mycoides cluster of ruminant pathogens, which vary widely in host range and pathobiology. Using (i) genome sequences from two members of this clade, Mycoplasma capricolum subsp. capricolum and M. mycoides subsp. mycoides small colony biotype (SC), (ii) antibodies to specific peptide determinants of predicted M. capricolum subsp. capricolum gene products, and (iii) analysis of the membrane-associated proteome of M. capricolum subsp. capricolum, a novel set of six genes (vmcA to vmcF) expressing distinct Vmc (variable M. capricolum subsp. capricolum) lipoproteins is demonstrated. These occur at two separate loci in the M. capricolum subsp. capricolum genome, which shares striking overall similarity and gene synteny with the M. mycoides subsp. mycoides SC genome. Collectively, Vmc expression is noncoordinate and combinatorial, subject to a single-unit insertion/deletion in a 5' flanking dinucleotide repeat that governs expression of each vmc gene. All vmc genes share modular regions affecting expression and membrane translocation. In contrast, vmcA to vmcD genes at one locus express surface proteins with highly structured size-variable repeating domains, whereas vmcE to vmcF genes express products with short repeats devoid of predicted structure. These genes confer a distinctive, dynamic surface architecture that may represent adaptive differences within this important group of pathogens as well as exploitable diagnostic targets.

Published

2006

26. U1 RNA induces innate immunity signaling.

Author

Hoffman RW, Gazitt T, Foecking MF, Ortmann RA, Misfeldt M, Jorgenson R, Young SL, and Greidinger EL

Subjects

Animals, Cell Division immunology, Cell Line, Humans, Interleukin-6 biosynthesis, Interleukin-6 immunology, Interleukin-8 biosynthesis, Interleukin-8 immunology, Ligands, Mice, Mice, Inbred C57BL, Mice, Knockout, Ribonucleoprotein, U1 Small Nuclear immunology, Toll-Like Receptor 3, Toll-Like Receptor 5, Toll-Like Receptors, Immunity, Innate immunology, Membrane Glycoproteins immunology, RNA, Small Nuclear immunology, Receptors, Cell Surface immunology, Signal Transduction immunology

Abstract

Objective: The U1-70-kd RNP is a prominent target of autoimmunity in connective tissue diseases. In this study, we explored whether its endogenous ligand, U1 RNA, mediates a proimmune signal and may be immunogenic., Methods: We assayed the proliferation of control and MyD88-knockout splenocytes in response to in vitro-synthesized U1 RNA, and measured interleukin-6 (IL-6) and IL-8 secretion induced by U1 RNA in a human cell line competent for signaling through Toll-like receptor 3 (TLR-3) and TLR-5., Results: Treatment with U1 RNA or with poly(I-C), a known agonist of TLR-3, induced approximately twice as much control splenocyte proliferation as did treatment with RNase-digested U1 RNA. Proliferation in response to either poly(I-C) or U1 RNA by MyD88-knockout splenocytes was similarly attenuated. Similar to poly(I-C), U1 RNA induced significant secretion of both IL-6 and IL-8 from a TLR-3-expressing human cell line; in contrast, the TLR-5 agonist flagellin induced predominantly IL-8 secretion. Pretreatment of U1 RNA with RNase abolished IL-6 and IL-8 secretion., Conclusion: U1 RNA is capable of inducing manifestations consistent with TLR-3 activation. The ability of U1 RNA (which has a substantial double-stranded secondary structure) to activate TLR-3 may contribute to the immunogenicity of the U1-70-kd autoantigen. Stimulation of innate immunity by native RNA molecules with a double-stranded secondary structure may help explain the high prevalence of autoimmunity to RNA binding proteins.

Published

2004

27. A major B cell epitope present on the apoptotic but not the intact form of the U1-70-kDa ribonucleoprotein autoantigen.

Author

Greidinger EL, Foecking MF, Magee J, Wilson L, Ranatunga S, Ortmann RA, and Hoffman RW

Subjects

Animals, Apoptosis genetics, Autoantibodies biosynthesis, Autoantibodies blood, Autoantigens administration & dosage, Autoantigens genetics, Autoantigens immunology, B-Lymphocytes immunology, Epitope Mapping, Epitopes, B-Lymphocyte administration & dosage, Epitopes, B-Lymphocyte genetics, Epitopes, B-Lymphocyte immunology, Humans, Immune Sera metabolism, Jurkat Cells, Lupus Erythematosus, Cutaneous pathology, Mice, Mice, Inbred C57BL, Mice, Knockout, Mice, Transgenic, Protein Structure, Tertiary, RNA-Binding Proteins administration & dosage, RNA-Binding Proteins genetics, RNA-Binding Proteins immunology, Ribonucleoprotein, U1 Small Nuclear administration & dosage, Ribonucleoprotein, U1 Small Nuclear genetics, Ribonucleoprotein, U1 Small Nuclear immunology, Vaccination, Apoptosis immunology, Autoantigens metabolism, B-Lymphocytes metabolism, Epitopes, B-Lymphocyte metabolism, Lupus Erythematosus, Cutaneous immunology, Ribonucleoprotein, U1 Small Nuclear metabolism

Abstract

Apoptotically modified forms of autoantigens have been hypothesized to participate in lupus immunopathogenesis. This study identifies a major B cell epitope present on the apoptotic but not the intact form of the U1-70-kDa ribonucleoprotein lupus autoantigen (70k). Human autoimmune sera with strong recognition of apoptotic 70k and minimal recognition of intact 70k were identified and tested for reactivity to truncated forms of 70k by immunoblot and ELISA. Patient sera that preferentially recognized apoptotic 70k were specific for an epitope dependent on residues 180-205 of the protein. This epitope was also recognized by 19 of 28 (68%) intact anti-70k-positive autoimmune human sera with Abs also recognizing apoptotic but not the intact form 70k, but only 1 of 9 (11%) intact 70k-positive sera without such Abs (Fisher's exact, p = 0.0055). Immunization of HLA-DR4-transgenic C57BL/6 mice with a peptide containing this epitope induced anti-70k immunity in 13 of 15 mice, including Abs recognizing apoptotic but not intact forms of autoantigens in 12 of 15 mice. Anti-70k responder mice also developed spreading of immunity to epitopes on the endogenous form of 70k, and proliferative lung lesions consistent with those described in patients with anti-70k autoimmunity. Thus, a major epitope in the B cell response to U1-70 kDa localizes to the RNA binding domain of the molecule, overlaps with the most common T cell epitope in the anti-70k response, and is not present on the intact form of the 70k molecule. Immunization of mice against this epitope induces an immune response with features seen in human anti-70k autoimmune disease.

Published

2004

28. T cell immunity in connective tissue disease patients targets the RNA binding domain of the U1-70kDa small nuclear ribonucleoprotein.

Author

Greidinger EL, Foecking MF, Schäfermeyer KR, Bailey CW, Primm SL, Lee DR, and Hoffman RW

Subjects

Alanine genetics, Amino Acid Sequence, Blood Donors, Clone Cells, Connective Tissue Diseases genetics, Epitopes, T-Lymphocyte genetics, Epitopes, T-Lymphocyte immunology, HLA-DR Antigens genetics, HLA-DRB1 Chains, Histocompatibility Testing, Humans, Molecular Sequence Data, Mutagenesis, Site-Directed, Peptide Fragments genetics, Peptide Fragments immunology, Peptide Fragments metabolism, Peptide Mapping, Protein Binding immunology, Protein Structure, Tertiary genetics, RNA, Small Nuclear immunology, RNA-Binding Proteins genetics, RNA-Binding Proteins metabolism, Ribonucleoprotein, U1 Small Nuclear genetics, Ribonucleoprotein, U1 Small Nuclear metabolism, Sequence Homology, Amino Acid, Connective Tissue Diseases immunology, RNA-Binding Proteins immunology, Ribonucleoprotein, U1 Small Nuclear immunology, T-Lymphocyte Subsets immunology

Abstract

Although the T cell dependence of autoimmune responses in connective tissue diseases has been well established, limited information exists regarding the T cell targeting of self Ags in humans. To characterize the T cell response to a connective tissue disease-associated autoantigen, this study generated T cell clones from patients using a set of peptides encompassing the entire linear sequence of the 70-kDa subunit of U1 snRNP (U1-70kDa) small nuclear ribonucleoprotein. Despite the ability of U1-70kDa to undergo multiple forms of Ag modification that have been correlated with distinct clinical disease phenotypes, a remarkably limited and consistent pattern of T cell targeting of U1-70kDa was observed. All tested T cell clones generated against U1-70kDa were specific for epitopes within the RNA binding domain (RBD) of the protein. High avidity binding of the RBD with U1-RNA was preserved with the disease-associated modified forms of U1-70kDa tested. The high avidity interaction between the U1-RBD on the polypeptide and U1-RNA may be critical in immune targeting of this region in autoimmunity. The T cell autoimmune response to U1-70kDa appears to have less diversity than is seen in the humoral response; and therefore, may be a favorable target for therapeutic intervention.

Published

2002

29. Apoptotic U1-70 kd is antigenically distinct from the intact form of the U1-70-kd molecule.

Author

Greidinger EL, Foecking MF, Ranatunga S, and Hoffman RW

Subjects

Antibody Specificity, Caspase 3, Caspases metabolism, Enzyme-Linked Immunosorbent Assay, Epitopes, B-Lymphocyte immunology, Humans, Protein Processing, Post-Translational immunology, Ribonucleoprotein, U1 Small Nuclear metabolism, Apoptosis immunology, Autoantigens immunology, Ribonucleoprotein, U1 Small Nuclear immunology

Abstract

Objective: To determine whether immune responses to an apoptotically modified form of a human lupus autoantigen can be distinguished from immune responses to the intact form of the same antigen., Methods: Immunoblot and enzyme-linked immunosorbent assay techniques were used to test human autoimmune sera for the presence of antibodies to apoptotic forms of the U1- 70-kd small nuclear RNP antigen, while antibody recognition of intact U1-70 kd was blocked., Results: poptosis-specific U1-70-kd antibodies were identified by immunoblot in 15 of 29 sera with antibodies to intact U1-70 kd and in 2 of 25 sera without measurable antibodies to intact U1-70 kd. Bacterially produced, purified, caspase-cleaved U1-70 kd without additional posttranslational modifications was a target of apoptosis-specific antibodies in 3 of 9 U1-70-kd-positive sera tested., Conclusion: The apoptotic form of U1-70 kd displays B cell epitopes that are not displayed on the intact form of U1-70 kd. Caspase cleavage in the absence of additional posttranslational modifications is sufficient to induce the display of some of these epitopes. Immunity to apoptotically modified proteins can develop against caspase-cleaved forms or against forms that undergo additional posttranslational modification.

Published

2002

30. Gas chromatography/mass spectrometry characterization of corticosteroid metabolism in human immortalized keratinocytes.

Author

Slominski A, Wortsman J, Foecking MF, Shackleton C, Gomez-Sanchez C, and Szczesniewski A

Subjects

Cell Line, Transformed, Chromatography, High Pressure Liquid, Chromatography, Thin Layer, Gas Chromatography-Mass Spectrometry, Humans, Progesterone metabolism, Desoxycorticosterone metabolism, Keratinocytes metabolism

Abstract

To continue our studies on the cutaneous expression of a proopiomelanocortin/corticotropin-releasing hormone system, we investigated whether this is accompanied by adrenal-type enzymatic activity. Immortalized cultured human keratinocytes were incubated with radiolabeled corticosteroids. Analysis by thin-layer chromatography showed rapid transformation of both progesterone and deoxycorticosterone; one of the progesterone metabolites migrated at the same rate as deoxycorticosterone. Gas chromatography/mass spectrometry further identified as major species of deoxycorticosterone metabolites 3beta,6alpha,21-trihydroxy-5alpha-pregnan-20-one, 3alpha,6alpha,21-trihydroxy-5alpha-pregnan-20-one, and 3alpha5alpha- and 3beta5alpha-tetrahydrodeoxycorticosterone. Minor metabolites were 3alpha,21-dihydroxy-5-pregnen-20- one (3alphaDelta5-21-OHpregnenolone), 3beta,21-dihydroxy-5-pregnen-20-one (3betaDelta5-21-OHpregnenolone), 3alpha,21-dihydroxy-4-pregnen-20-one (3alphaDelta4-21-OHpregnenolone), 6-hydroxy-dihydrodeoxycorticosterone, and two 5-dihydrodeoxycorticosterone species. Thus, in addition to sex steroids keratinocytes also actively metabolize corticosteroids along similar enzymatic pathways. The surprising detection of 3alphaDelta5-21-OHpregnenolone and 3 betaDelta5-21-OHpregnenolone, indicating Delta4-ketosteroids to Delta5-hydroxysteroids conversion, provides strong evidence for the occurrence, at least in human keratinocytes, of isomerase activity that allows the reaction to proceed in reverse of its usual direction. As skin expresses 3alpha/beta-hydroxysteroid dehydrogenase/Delta5-Delta4 isomerases, cutaneous reactions catalyzed by these enzymes must be reversible. In conclusion, besides elements of the corticotropin-releasing hormone/proopiomelanocortin system human keratinocytes show high levels of corticosteroid metabolizing activity. Moreover, the wide array of steroid products generated from a single substrate indicates serial progressive conversion involving 5alpha-reductase, 6alpha-hydroxylase, 3alpha/beta-hydroxysteroid dehydrogenase, and reverse Delta4minus signDelta5 isomerase enzymes. As distinct from the adrenal cortex, production of A, B, Aldo, 18OHdeoxycorticosterone, or F in keratinocytes was absent or below limits of detectability.

Published

2002

31. Serum 18-hydroxycortisol in primary aldosteronism, hypertension, and normotensives.

Author

Mosso L, Gómez-Sánchez CE, Foecking MF, and Fardella C

Subjects

Adult, Cytochrome P-450 CYP11B2 genetics, Enzyme-Linked Immunosorbent Assay, Female, Humans, Hyperaldosteronism genetics, Hypertension genetics, Male, Middle Aged, Steroid 11-beta-Hydroxylase genetics, Hydrocortisone analogs & derivatives, Hydrocortisone blood, Hyperaldosteronism blood, Hypertension blood

Abstract

This study reports the determination of plasma 18-hydroxycortisol (18-OHF) using a new and easy enzyme-linked immunosorbent assay (ELISA) method in primary aldosteronism and compares the values found in essential hypertensives and normotensive controls. In primary aldosteronism, we evaluated usefulness of plasma 18-OHF determination and the dexamethasone suppression test in the diagnosis of glucocorticoid-remediable aldosteronism using the genetic test as the gold standard. We studied 31 primary aldosteronism patients, 101 essential hypertensives, and 102 healthy normotensive controls. The plasma 18-OHF was measured using a biotin-avidin enzyme-linked assay by a new and purified polyclonal antibody. The 18-OHF value in primary aldosteronism was 6.3+/-8.05 nmol/L; this value is significantly higher than the value found in essential hypertensives and normotensive controls (2.81+/-1.42 and 2.70+/-1.41 nmol/L, respectively; P<0.0005). In primary aldosteronism, 4 of 31 patients had 18-OHF levels that were 10 times higher than the normal upper limit (2.983 nmol/L). The dexamethasone suppression test in primary aldosteronism patients was positive (serum aldosterone <4 ng/dL) in 13 of 31 cases. A chimeric CYP11B1/CYP11B2 gene was demonstrated in 4 primary aldosteronism patients, corresponding to the same cases that had higher level of 18-OHF. In conclusion, plasma 18-OHF determination by this ELISA method is reliable for detecting glucocorticoid-remediable aldosteronism, and it does so better than the dexamethasone suppression test.

Published

2001

32. Steroidogenesis in the human skin: 21-hydroxylation in cultured keratinocytes.

Author

Rogoff D, Gomez-Sanchez CE, Foecking MF, Wortsman J, and Slominski A

Subjects

Adrenal Glands metabolism, Cell Line, Cells, Cultured, Chromatography, Thin Layer, Desoxycorticosterone metabolism, Estrogens metabolism, Humans, Kinetics, Microsomes metabolism, Polymerase Chain Reaction, Progesterone metabolism, RNA, Messenger metabolism, Reverse Transcriptase Polymerase Chain Reaction, Keratinocytes metabolism, Skin metabolism, Steroid 21-Hydroxylase metabolism

Abstract

We have evaluated the metabolism of radiolabeled progesterone (P) by the microsomal fraction isolated from HaCaT keratinocytes. P was widely metabolized to different compounds that included DOC (5-7% conversion) thus demonstrated 21-hydroxylase (21-OHase) activity, a key step in adrenal synthesis of gluco- and mineralocorticoids. However, RT-PCR amplification for the CYPc21 transcript of the corresponding gene showed no evidence for gene expression in HaCaT cells suggesting that the 21-OHase enzyme present in keratinocytes is different from that described in adrenal gland. Further characterization showed that whereas estradiol stimulated markedly P metabolism by HaCaT microsomes, with generation of new unidentified compounds, Lineweaver-Burk analysis of keratinocyte 21-OHase activity showed that the K(m) and V(max) were unaffected by estrogen. The apparent K(m) was 0.6 microM without estradiol and 0.7 microM with estradiol, while the respective V(max) values were 60 and 76 nmol/l/min. To conclude, we found extensive metabolism of P in human keratinocytes, we also provide the first demonstration of 21-OHase activity in this cell system and further showed that it is coded by a gene different from the adrenal CYPc21.

Published

2001

33. Aldosterone esters and the heart.

Author

Gomez-Sanchez CE, Foecking MF, and Gomez-Sanchez EP

Subjects

Animals, Blood metabolism, Chromatography, High Pressure Liquid, Chromatography, Thin Layer, Enzyme-Linked Immunosorbent Assay, Esters, Hydrolysis, In Vitro Techniques, Radioimmunoassay, Rats, Rats, Sprague-Dawley, Aldosterone analogs & derivatives, Aldosterone metabolism, Myocardium metabolism

Abstract

There are clinical and experimental situations in which symptoms of mineralocorticoid excess are remediable with mineralocorticoid receptor antagonist treatment, in spite of paradoxically low levels of plasma renin and aldosterone. Several decades ago, a factor isolated from the heart was described that had mineralocorticoid properties like those of aldosterone, but much more potent. It was thought to be similar to aldosterone-18-monoacetate or -21-monoacetate, acetyl derivatives of aldosterone that are very rapidly hydrolyzed in the circulation. In our efforts to confirm and extend these observations, we extracted rat hearts and plasma harvested in a manner that would minimize hydrolysis. The product was subjected to several forms of TLC and HPLC and compared to several acetylated derivatives of aldosterone standards. We found that 68% of the aldosterone extracted from fresh myocardium corresponded to an aldosterone derivative that migrates at the same rate as aldosterone-20-monoacetate. The identity of this compound awaits definitive analysis. Tritiated aldosterone-21-monoacetate hydrolyzed to form aldosterone very rapidly; negligible monoacetate remained in blood left at 37 degrees C for 5 min or in hearts left at room temperature for 30 min. Regulation of aldosterone production serves the requirements of fluid and electrolyte homeostasis provided by transport epithelia, primarily that of the kidney. Nonepithelial actions of aldosterone would be freed of these regulatory constraints if the formation of a more potent derivative of the parent compound to which it is almost immediately hydrolyzed in the circulation were regulated within the nonepithelial target tissues.

Published

2001

34. Active steroidogenesis in the normal rat skin.

Author

Slominski A, Gomez-Sanchez CE, Foecking MF, and Wortsman J

Subjects

Animals, Autoradiography, Carbon Radioisotopes, Chromatography, Thin Layer, Corticosterone biosynthesis, Desoxycorticosterone biosynthesis, Desoxycorticosterone metabolism, Male, Progesterone metabolism, Rats, Rats, Inbred Dahl, Skin metabolism, Steroids biosynthesis

Abstract

Using the radiolabeled precursors of adrenal steroids (14)C-11-deoxycorticosterone (DOC) and (14)C-progesterone ((14)C-PROG) we demonstrate that rat skin can synthesize a number of steroids. TLC separation of labeled metabolites show that among the (14)C-steroid products, two co-migrate with corticosterone (B) and 11-dehydrocorticosterone (A) standards. Thus, normal rodent skin possesses steroidogenic activity that can be shown using progesterone or DOC as primary substrates.

Published

2000

35. Metabolism of progesterone to DOC, corticosterone and 18OHDOC in cultured human melanoma cells.

Author

Slominski A, Gomez-Sanchez CE, Foecking MF, and Wortsman J

Subjects

Adrenal Glands metabolism, Adrenocorticotropic Hormone pharmacology, Aldosterone biosynthesis, Angiotensin II pharmacology, Humans, Kinetics, Skin metabolism, Tumor Cells, Cultured, Corticosterone biosynthesis, Desoxycorticosterone analogs & derivatives, Desoxycorticosterone biosynthesis, Melanoma metabolism, Progesterone metabolism

Abstract

We are now showing that cultured human melanoma cells can synthesize steroids such as corticosterone from progesterone or deoxycorticosterone. Corticosterone production is strongly responsive to deoxycorticosterone substrate addition (12-fold increase), but unresponsive to the adrenal stimulating factors ACTH and angiotensin II. This is the first demonstration that skin cells (malignant melanocytes) have the capability to synthesize 11-deoxycorticosterone, corticosterone, and 18-hydroxydeoxycorticosterone.

Published

1999

36. Aldosterone biosynthesis in the rat brain.

Author

Gomez-Sanchez CE, Zhou MY, Cozza EN, Morita H, Foecking MF, and Gomez-Sanchez EP

Subjects

Animals, Blotting, Southern, Brain drug effects, Brain enzymology, Brain Chemistry, Chromatography, High Pressure Liquid, Corticosterone antagonists & inhibitors, Corticosterone metabolism, Cytochrome P-450 CYP11B2 analysis, Cytochrome P-450 CYP11B2 genetics, Cytochrome P-450 CYP11B2 physiology, DNA Primers analysis, DNA Primers chemistry, DNA Primers genetics, Desoxycorticosterone pharmacology, Enzyme-Linked Immunosorbent Assay, Female, Hydrocortisone pharmacology, Male, Metyrapone pharmacology, Mineralocorticoid Receptor Antagonists pharmacology, Polymerase Chain Reaction, RNA, Messenger analysis, RNA, Messenger chemistry, RNA, Messenger genetics, Rats, Rats, Sprague-Dawley, Aldosterone biosynthesis, Brain metabolism

Abstract

Messenger RNA (mRNA) for enzymes involved in adrenal steroid biosynthesis are expressed in the brain, and the coded enzymes have been shown to be active. The expression of mRNA for the cytochrome P-450 enzyme aldosterone synthase, crucial for the final step in the synthesis of aldosterone and the synthesis of aldosterone was studied in several anatomic areas of the rat brain. Expression of the mRNA for the aldosterone synthase was demonstrated by RT-PCR/Southern blot in adrenal, aorta, hypothalamus, hippocampus, amygdala, cerebrum, and cerebellum. Incubation of brain minces from intact and adrenalectomized rats demonstrated the synthesis of corticosterone and aldosterone from endogenous precursors. Incubations of brain minces with [1,2(3)H]-deoxycorticosterone, followed by extraction and three different successive TLCs, demonstrated the presence of labeled aldosterone, corticosterone, and 18-hydroxy-deoxycorticosterone. Incubation, in the presence of 10 microM cortisol or metyrapone, inhibited the synthesis of aldosterone or both aldosterone and corticosterone, respectively. These studies indicate that the rat brain has the enzymatic machinery for the synthesis of adrenal corticosteroids and is capable of synthesizing aldosterone. Aldosterone synthesized in the brain might play a paracrine role in the regulation of blood pressure.

Published

1997

37. Inhibition of steroidogenesis in rat adrenal cells by 18-ethynyldeoxycorticosterone: evidence for an alternative pathway of aldosterone biosynthesis.

Author

Gomez-Sanchez CE, Gomez-Sanchez EP, Foecking MF, and Zhou MY

Subjects

Animals, Cells, Cultured, Desoxycorticosterone pharmacology, Rats, Rats, Sprague-Dawley, Adrenal Glands metabolism, Aldosterone biosynthesis, Desoxycorticosterone analogs & derivatives

Abstract

The effect of the mechanism-based inhibitor 18-ethynyldeoxycorticosterone (18-E-DOC) on the late steps of the aldosterone biosynthetic pathway was examined in freshly isolated cells of the zona glomerulosa (ZG) and fasciculata (ZF) from rat adrenal glands. ZG synthesis of aldosterone was inhibited by 18-E-DOC in a time- and concentration-dependent manner with a Ki of approximately 0.05 microM. The maximal degree of inhibition of ZG production of aldosterone and 18-hydroxycorticosterone (18-OH-B) was approximately 80%. ZF cells, perhaps surprisingly, were found to secrete 18-OH-B at levels approximately one-third to one-fourth those of ZG cells and the Ki of 18-E-DOC inhibition of 18-OH-B secretion was approximately 10 microM for ZF cells, 200-fold higher than for ZG cells. The inhibitor had no effect on the secretion of corticosterone by either ZG or ZF, and the secretion of 18-hydroxydeoxycorticosterone (18-OH-DOC) by both the ZG and ZF was inhibited only to a minor degree. 18-E-DOC inhibited the biosynthesis of aldosterone by ZG cells incubated with 10 microM added DOC or 18-OH-DOC by approximately 75%, similar to the degree of inhibition of aldosterone biosynthesis from endogenous substrate, whereas ZF biosynthesis of 18-OH-B from either substrate was inhibited by less than 40%. ZF cells do not express aldosterone synthase, the only enzyme known to convert 18-OH-DOC into 18-OH-B. Incubation of MA-10 cells stably transfected with the cDNA of the rat aldosterone synthase with 18-E-DOC resulted in a complete inhibition of the conversion of DOC to aldosterone with a Ki of approximately 0.02 microM. In addition, transfected cells expressing 11beta-hydroxylase convert DOC to 18-OH-B in very small quantities only and cannot convert 18-OH-DOC to 18-OH-B. These data suggest that neither 11beta-hydroxylase nor aldosterone synthase are responsible for the biosynthesis of 18-OH-B by ZF cells from DOC or 18-OH-DOC, that 20% of aldosterone synthesis appears not to be attributable to the actions of aldosterone synthase and that an unknown CYP11B enzyme is also involved in the biosynthesis of 18-OH-B.

Published

1997

38. Mutations in the 11 beta-hydroxylase genes in the Dahl SS and SR rats.

Author

Gomez-Sanchez EP, Zhou M, Morita H, Cozza EN, Foecking MF, and Gomez-Sanchez CE

Subjects

Animals, Corticosterone biosynthesis, Cytochrome P-450 CYP11B2 genetics, DNA, Complementary, Desoxycorticosterone metabolism, Rats, Rats, Mutant Strains, Transfection, Hypertension enzymology, Mutation, Steroid 11-beta-Hydroxylase genetics

Published

1996

39. 11 beta-Hydroxysteroid dehydrogenase type 2 complementary deoxyribonucleic acid stably transfected into Chinese hamster ovary cells: specific inhibition by 11 alpha-hydroxyprogesterone.

Author

Morita H, Zhou M, Foecking MF, Gomez-Sanchez EP, Cozza EN, and Gomez-Sanchez CE

Subjects

11-beta-Hydroxysteroid Dehydrogenases, Animals, Corticosterone analogs & derivatives, Corticosterone metabolism, Cricetinae, Dexamethasone metabolism, Female, Humans, Hydroxyprogesterones urine, Hydroxysteroid Dehydrogenases genetics, Hydroxysteroid Dehydrogenases metabolism, Kidney ultrastructure, Male, Microsomes enzymology, NAD pharmacology, Pregnancy, Rats, CHO Cells enzymology, DNA, Complementary genetics, Enzyme Inhibitors pharmacology, Hydroxyprogesterones pharmacology, Hydroxysteroid Dehydrogenases antagonists & inhibitors, Transfection

Abstract

The 11 beta-hydroxysteroid dehydrogenase type 2 (11 beta HSD-2) enzyme is thought to confer aldosterone specificity upon mineralocorticoid target tissues by protecting the mineralocorticoid receptor from binding by the more abundant glucocorticoids, corticosterone and cortisol. We have developed a Chinese hamster ovary cell line stably transfected with a plasmid containing the rat 11 beta HSD-2 complementary DNA. This cell line has expressed the enzyme consistently for many generations. The 11 beta HSD-2 was located primarily in the microsomes, but significant amounts also existed in the nuclei and mitochondria. The enzymatic reaction was unidirectional, oxidative, and inhibited by the product, 11-dehydrocorticosterone, with an IC50 of approximately 200 nM. The K(m) for corticosterone was 9.6 +/- 3.1 nM, and that for NAD+ was approximately 8 microM. The enzyme did not convert dexamethasone to 11-dehydrodexamethasone. Tunicamycin, an N-glycosylation inhibitor, had no effect on enzyme activity. 11 alpha-Hydroxyprogesterone (11 alpha OH-P) was an order of magnitude more potent a competitive inhibitor of the 11 beta HSD-2 than was glycyrrhetinic acid (GA) (approximate IC50 = 0.9 vs. 15 nM). 11 beta OH-P, progesterone, and GA were almost equipotent (IC50 = 10 and 6 nM, respectively), and 5 alpha-pregnandione and 5 beta-pregnandione were less potent (IC50 = 100 and 500 nM, respectively) inhibitors of the enzyme. When the inhibitory activities were examined with intact transfected cells, 11 alpha OH-P was more potent than GA (IC50 = 5 and 150 nM, respectively). 11 alpha OH-P was not metabolized by 11 beta HSD-2. We were unable to demonstrate the presence of 11 alpha OH-P in human urine. In conclusion, a cell line stably transfected with the rat 11 beta HSD-2 was created, and the enzyme kinetics, including inhibition, were characterized. 11 alpha OH-P was found to be a potent relatively specific inhibitor of the 11 beta HSD-2 enzyme. Its potential importance is that it is the most specific inhibitor of the 11 beta HSD-2 so far encountered and would aid in the study of the physiological importance of the isoenzyme.

Published

1996

40. Cloning and expression of the rat adrenal cytochrome P-450 11B3 (CYP11B3) enzyme cDNA: preferential 18-hydroxylation over 11 beta-hydroxylation of DOC.

Author

Zhou MY, Gomez-Sanchez EP, Foecking MF, and Gomez-Sanchez CE

Subjects

Adrenal Glands enzymology, Amino Acid Sequence, Animals, Animals, Newborn, Base Sequence, Brain enzymology, Cell Line, Cloning, Molecular, Cytochrome P-450 CYP11B2, Cytochrome P-450 Enzyme System metabolism, DNA Primers genetics, Desoxycorticosterone chemistry, Desoxycorticosterone metabolism, Gene Expression, Hydroxylation, Molecular Sequence Data, Point Mutation, Polymerase Chain Reaction, RNA, Messenger genetics, RNA, Messenger metabolism, Rats, Steroid 11-beta-Hydroxylase metabolism, Transfection, Cytochrome P-450 Enzyme System genetics, DNA, Complementary genetics, Steroid 11-beta-Hydroxylase genetics

Abstract

The biosynthesis of glucocorticoids and mineralocorticoids in the rat adrenal cortex requires the action of two different cytochrome P450 11 beta-hydroxylases, CYP11B1 and CYP11B2, which are distributed in the zona fasciculata and glomerulosa, respectively. The existence of another cytochrome P450-11 beta gene, CYP11B3, was recently reported. Although CYP11B3 has similar gene structure and great homology to the CYP11B1 and -B2 genes, the CYP11B3 mRNA was not originally detected by reverse transcription-polymerase chain reaction (RT-PCR) and has only recently been cloned and detected from neonatal rat adrenals. Herein we demonstrate RT-PCR detection of CYP11B3 mRNA expressed in adult rat adrenal and brain tissues. The whole coding region of the CYP11B3 enzyme cDNA was cloned and sequenced. When transiently expressed in COS-7 cells the CYP11B3 converted deoxycorticosterone (DOC) to corticosterone and 18-hydroxydeoxycorticosterone, but not to 18-hydroxycorticosterone or aldosterone. It produced more 18-OH-DOC than corticosterone. A single mutation in CYP11B3 in which Gly-59 was replaced by Ser, reduced the enzymatic activity 5-6-fold. Furthermore, CYP11B3 mRNA expression is greater in neonatal, compared to adult rat adrenal glands.

Published

1995

41. Stable expression of rat cytochrome P450 11 beta-hydroxylase (CYP11B1) and aldosterone synthase (CYP11B2) in MA-10 cells.

Author

Zhou M, Xue D, Foecking MF, and Gomez-Sanchez CE

Subjects

18-Hydroxycorticosterone metabolism, Adrenal Cortex enzymology, Animals, Cell Line, Corticosterone biosynthesis, Cytochrome P-450 CYP11B2, Cytochrome P-450 Enzyme System metabolism, DNA, Complementary genetics, Desoxycorticosterone metabolism, Gene Expression, Male, Rats, Steroid 11-beta-Hydroxylase metabolism, Transfection, Cytochrome P-450 Enzyme System genetics, Steroid 11-beta-Hydroxylase genetics

Abstract

Glucocorticoids and mineralocorticoids are synthesized in the adrenal cortex through the action of two different cytochrome 11 beta-hydroxylases, CYP11B1 (11 beta-hydroxylase) and CYP11B2 (aldosterone synthase) which are distributed in the zona fasciculata and glomerulosa, respectively. We have created stably transfected cell lines using the Leydig tumor cell line MA-10 with CYP11B1 and CYP11B2 cDNA-containing plasmids which have a selectable gene to confer resistance to geneticin. The expression of the transfected cDNA in the cells was characterized by Northern-blot and measurement of enzymatic activity. The cell lines express the enzymes stably for many generations. CYP11B1 transfected cells converted DOC into corticosterone, 18-OH-DOC and small amounts of 18-OH-corticosterone, in a time and concentration dependent manner. Incubation of the cells with corticosterone generated 18-OH-corticosterone especially at concentrations of 30 and 100 microM. The production of 18-OH-corticosterone from corticosterone at these doses was significantly higher than incubations with similar concentrations of DOC. CYP11B2 transfected cells converted DOC into corticosterone, 18-OH-corticosterone, aldosterone and small amounts of 18-OH-DOC in a time and concentration dependent manner. They converted corticosterone into 18-OH-corticosterone and aldosterone in a time and concentration dependent manner. The absolute and relative production of aldosterone from DOC was significantly higher than when cells were incubated with corticosterone, and the ratio of aldosterone to 18-OH-corticosterone was higher at all concentrations of DOC compared to corticosterone. CYP11B2 transfected cells (but not the CYP11B1 transfected cells) transform 18-OH-DOC into 18-OH-corticosterone, but can not convert 18-OH-DOC into aldosterone. In conclusion, stably transfected MA-10 cells with the cDNAs for the CYP11B1 and CYP11B2 enzymes were prepared and their enzymatic activity studied. These cells are useful in the study of inhibitors of the specific enzymes, as well as determining the roles that each enzyme plays in zone-specific steroidogenesis in the adrenal cortex.

Published

1995

42. Is the circulating ouabain-like compound ouabain?

Author

Gomez-Sanchez EP, Foecking MF, Sellers D, Blankenship MS, and Gomez-Sanchez CE

Subjects

Adrenal Glands chemistry, Adrenal Glands cytology, Animals, Cattle, Chromatography, High Pressure Liquid, Enzyme-Linked Immunosorbent Assay, Humans, Ouabain analysis, Rabbits, Rats, Rats, Inbred Strains, Tissue Extracts chemistry, Ouabain blood, Ouabain chemistry

Abstract

The evidence is very strong for a circulating inhibitor of the sodium, potassium ATPase in volume-expanded hypertension. Recently, this inhibitor was isolated from human plasma and identified as ouabain. We are reporting our results using a very specific and sensitive immunoassay for ouabain with which we were unable to detect or able to detect only very low levels of circulating immunoreactive ouabain. Immunoassay of 5 mL of human and rat plasma, incubation fluid from bovine and human adrenal cell cultures extracted using a C-18 solid phase column, and HPLC separation did not detect a peak corresponding to ouabain. This procedure could easily detect authentic ouabain added to these extracts at a concentration slightly below that reported to be present by others. The extract from the adrenal cultures had clearly detectable sodium, potassium ATPase using an assay based on inhibition of tritiated ouabain binding to human red cells. Extraction of bovine adrenals detected a very small amount of immunoassayable ouabain which did not elute at a time corresponding to that of ouabain. This study indicates that the postulated sodium, potassium ATPase inhibitor that circulates in plasma is not ouabain, but it is likely to be structurally similar to ouabain, as it appears to cross-react with some antibodies against ouabain.

Published

1994

43. The hybrid rat cytochrome P450 containing the first 5 exons of the CYP11B1 and last 4 exons from the CYP11B2 enzyme retains 11 beta-hydroxylase activity, but the alternative hybrid is inactive.

Author

Zhou MY, Gomez-Sanchez CE, Xue D, and Foecking MF

Subjects

Animals, Base Sequence, Cytochrome P-450 CYP11B2, Molecular Sequence Data, Rats, Recombinant Fusion Proteins metabolism, Structure-Activity Relationship, Substrate Specificity, Cytochrome P-450 Enzyme System chemistry, Steroid 11-beta-Hydroxylase chemistry

Abstract

Human, mouse and rats have 2 different cytochrome P-450 11 beta-hydroxylases in the adrenal cortex. The classical rat 11 beta-hydroxylase or CYP11B1 enzyme hydroxylates deoxycorticosterone to corticosterone and 18-hydroxydeoxycorticosterone and is located throughout the adrenal. The second aldosterone synthase or CYP11B2 enzyme is located in the zona glomerulosa and converts deoxycorticosterone to corticosterone, 18-hydroxycorticosterone and aldosterone. In rat the coding nucleotide sequence and the deduced amino acid sequences of the CYP11B1 and CYP11B2 genes are homologous by 88% and 83%, respectively. We have constructed two different hybrid cDNAs by exchanging two fragments of the rat CYP11B1 and CYP11B2 at the junction of the 5/6 exon and expressed them in COS 7 cells. The hybrid CYPH11B1 construct containing the first 5 exons of the CYP11B1 when expressed, retains 11 beta-hydroxylase activity, but cannot process corticosterone to 18-hydroxycorticosterone or aldosterone. The hybrid CYPH11B2 construct containing the first 5 exons of the CYP11B2 enzyme when expressed is inactive.

Published

1994

44. Synthesis of 18-hydroxycortisol and 18-oxocortisol in bovine adrenal zona glomerulosa mitochondria.

Author

Cozza EN, Chavarri MR, Foecking MF, and Gomez-Sanchez CE

Subjects

18-Hydroxycorticosterone metabolism, Aldosterone metabolism, Animals, Binding, Competitive, Cattle, Corticosterone metabolism, Corticosterone pharmacology, Dithionite pharmacology, Hydrocortisone biosynthesis, Hydrocortisone metabolism, Hydrocortisone pharmacology, Kinetics, Mitochondria drug effects, NADP pharmacology, Spectrophotometry, Zona Glomerulosa drug effects, Zona Glomerulosa metabolism, Hydrocortisone analogs & derivatives, Mitochondria metabolism, Zona Glomerulosa ultrastructure

Abstract

The biosynthesis of 18-hydroxycortisol and 18-oxocortisol from cortisol was studied in calf adrenal zona glomerulosa mitochondria. Cortisol is converted to 18-hydroxycortisol and 18-oxocortisol in the same mitochondrial preparation in which corticosterone is metabolized to 18-hydroxycorticosterone and aldosterone. Cortisol and 18-hydroxycortisol interacted with mitochondria to cause a Type I differential spectrum, which was decreased by sodium dithionite. The metabolism of cortisol to 18-hydroxycortisol and 18-oxocortisol was inhibited by metyrapone in a competitive way. Cortisol was a competitive inhibitor of the transformation of corticosterone into 18-hydroxycorticosterone and aldosterone, and corticosterone was a competitive inhibitor of the transformation of cortisol into 18-hydroxycortisol and 18-oxocortisol, with a Ki very similar to the Km for the transformation of that steroid to aldosterone. These results indicate that cortisol is metabolized to 18-hydroxycortisol and 18-oxocortisol by a mitochondrial cytochrome P-450, which is the same as that which catalyzes the conversion of corticosterone into aldosterone.

Published

1993

45. Adrenal receptors for natriuretic peptides and inhibition of aldosterone secretion in calf zona glomerulosa cells in culture.

Author

Cozza EN, Foecking MF, Vila MC, and Gomez-Sanchez CE

Subjects

Aldosterone biosynthesis, Animals, Cattle, Cells, Cultured, Cross-Linking Reagents, Natriuretic Peptide, Brain, Zona Glomerulosa cytology, Aldosterone metabolism, Nerve Tissue Proteins metabolism, Receptors, Atrial Natriuretic Factor metabolism, Receptors, Cell Surface metabolism, Zona Glomerulosa metabolism

Abstract

Atrial and brain natriuretic peptides specifically bind to primary cultures of calf adrenal glomerulosa cells. Binding of both natriuretic peptides to the same receptor has been proved by: a Dixon plot showing competitive effects for the binding of 125I-labeled brain natriuretic peptide in the presence of increasing concentrations of unlabeled atrial natriuretic peptide; a Scatchard plot showing a lower dissociation constant (Kd) for atrial natriuretic peptide than for brain natriuretic peptide binding, but the maximum binding (Bmax) values were the same; autoradiography of sodium dodecyl sulfate polyacrylamide gels after cross-linking of 125I-labeled atrial natriuretic peptide and 125I-labeled brain natriuretic peptide, showing the same molecular weights for both peptide receptors--a single 66-kD band in whole cells and a main band at 125 kD in membranes. C-Type atrial natriuretic peptide only slightly displaced atrial natriuretic peptide binding. Angiotensin II- and potassium-mediated stimulation of aldosterone production were inhibited strongly and to the same degree by atrial and brain natriuretic peptide but only slightly by C-type atrial natriuretic peptide. Stimulation of aldosterone production mediated by adrenocorticotropin was only partially inhibited by atrial and brain natriuretic peptide, while baseline aldosterone was not affected. These results suggest that atrial and brain natriuretic peptide bind to the same receptors and provoke the same effects on aldosterone production. The weak effects found with C-type atrial natriuretic peptide suggest that the primary culture of calf adrenal glomerulosa cells contain the guanylate cyclase A receptor.

Published

1993

46. Endothelin receptor subtypes and stimulation of aldosterone secretion.

Author

Gomez-Sanchez CE, Cozza EN, Foecking MF, Chiou S, and Ferris MW

Subjects

Animals, Binding, Competitive, Down-Regulation, Endothelins, Endothelium, Vascular, Peptides metabolism, Peptides pharmacology, Receptors, Cell Surface drug effects, Receptors, Endothelin, Vasoconstrictor Agents, Viper Venoms metabolism, Viper Venoms pharmacology, Aldosterone metabolism, Receptors, Cell Surface metabolism

Abstract

Endothelins (ETs) are 21-amino acid peptides with two disulfide bonds that have powerful vasoactive properties. We have previously shown the presence of a specific, high-affinity, saturable receptor for porcine or human endothelin (ET-1) in cultured calf zona glomerulosa cells. ET-1 was a stimulator of aldosterone secretion although not as powerful as angiotensin II. Incubations of cultured calf zona glomerulosa cells with Sarafotoxin S6b (S6b), a snake venom that has a structure highly homologous to ET-1, stimulated aldosterone secretion with a potency similar to that of ET-1. Binding of [125I]ET-1 to the adrenal receptor gave a Kd of 0.17 +/- 0.05 nM and a Bmax of 36 +/- 8.5 fmol/well (n = 4). Displacement of [125I]ET-1 by unlabeled ETs and S6b showed that the concentrations needed to displace 50% of the tracer were 0.3 nM for ET-1, 0.3 nM for ET-2, 10 nM for S6b, and 100 nM for ET-3. Binding of [125I]S6b to cultured adrenal cells revealed a receptor with a Kd of 0.05 +/- 0.01 nM and a Bmax of 8 +/- 2 fmol/well (n = 4). Displacement of [125I]S6b by unlabeled ETs and S6b showed that the concentrations needed to displace 50% of the tracer were 0.03 nM for S6b, 0.06 nM for ET-1, 0.04 nM for ET-2, and 0.05 nM for ET-3. Unlabeled ET-1 and ET-2 preferentially down-regulated the binding of [125I]ET-1, and S6b preferentially down-regulated the binding of [125I]S6b.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1990

47. The binding of cortisol to adrenal mitochondria.

Author

Cozza EN, Foecking MF, and Gómez-Sánchez CE

Subjects

Animals, Cattle, Corticosterone metabolism, Dithionite pharmacology, In Vitro Techniques, Temperature, Hydrocortisone metabolism, Mitochondria metabolism, Zona Glomerulosa metabolism

Abstract

Binding of tritiated cortisol to adrenal zona glomerulosa mitochondria was studied and compared with that of corticosterone. Cortisol was shown to bind specifically to the inner membrane of zona glomerulosa mitochondria. Corticosterone and cortisol had similar apparent association constants (Ka) and concentrations of binding sites. The methodology was validated by obtaining similar Ka from both binding plots and kinetic data. Cortisol binding was inhibited by pretreatment with sodium dithionite, and displaced by deoxycorticosterone, corticosterone, 18-hydroxy-corticosterone, 11 beta-hydroxy-18-ethynyl-progesterone and metyrapone, but not by cholesterol. These results suggest that cortisol and corticosterone bind to the same cytochrome P-450.

Published

1990

48. Rat mesenteric artery endothelial cells in culture secrete ET-1.

Author

Gomez-Sanchez CE, Foecking MF, Ferris MW, Hieda HS, and Gomez-Sanchez EP

Subjects

Cells, Cultured, Chromatography, High Pressure Liquid, Cross Reactions, Endothelins, Peptides immunology, Radioimmunoassay, Endothelium, Vascular metabolism, Mesenteric Arteries metabolism, Peptides metabolism

Abstract

Endothelial cells were harvested by the collagenase perfusion of isolated mesenteric arteries of rats and cultured. An endothelin peptide was detected in the supernatant of these cells by an antibody which recognizes ET-1 but not "rat" endothelin (ET-3). Culture media was extracted using a C-8 solid phase column and subjected to reverse phase HPLC using a system that separates all known endothelins and immunoreactive endothelins measured using another antibody which recognizes all endothelins. The main immunoreactive peak co-eluted with ET-1. We could not detect any ET-2, ET-3 or Vasoactive Intestinal Contractor. A smaller immunoreactive peak of unknown structure that eluted earlier than ET-1 was also detected. In conclusion, rat endothelial cells secrete a peptide of similar chromatographic and immunoreactive properties as ET-1.

Published

1990

49. The production of monoclonal antibodies against aldosterone.

Author

Gomez-Sanchez CE, Foecking MF, Ferris MW, Chavarri MR, Uribe L, and Gomez-Sanchez EP

Subjects

Animals, Antibodies, Monoclonal biosynthesis, Antibodies, Monoclonal isolation & purification, Antibody Specificity, Cross Reactions, Mice, Steroids immunology, Aldosterone immunology, Antibodies, Monoclonal immunology

Abstract

We have prepared several monoclonal antibodies against aldosterone-3-carboxy-methyloxime-BSA conjugate by fusing spleen lymphocytes from an immunized mouse with the mouse myeloma line HL-1 Friendly. A total of 6 different clones were isolated and expanded. All of the antibodies exhibited low cross-reactivities against most of the compounds tested. Antibodies A5A3, A2E11, and C1E2 exhibited low cross-reactivity with 18-hydroxycorticosterone and 18-hydroxydeoxycorticosterone and showed no detectable displacement of tritiated aldosterone from the antibodies with cortisol, corticosterone, and related steroids. The only steroid that showed moderate cross-reactivity was 3 alpha,5 beta-tetrahydroaldosterone (around 3%). Clone A5H12 antibodies exhibited high cross-reactivity with tetrahydroaldosterone (19.3%) but otherwise was very similar to the above clones. Antibody of clone C1E4 showed high cross-reactivity to tetrahydroaldosterone (41.2%) and 18-hydroxyDOC (2%) with relatively low cross-reactivity to DOC (0.078%). Clone A2G9 antibodies were the only ones for which cortisol and corticosterone displaced tritiated aldosterone with cross-reactivities of 0.0042% and 0.125%, making them unsuitable for a direct radioimmunoassay of plasma aldosterone. The monoclonal antibodies were very sensitive to freezing and thawing. The cross-reactivities of the first three clones' antibodies compare favorably with those polyclonal antibodies that have been described to be suitable for use in direct radioimmunoassays of plasma aldosterone. Their advantage is the reliable supply of an antibody with consistent, predictable properties.

Published

1987

50. 18-Hydroxy-11-deoxycortisol: a new steroid isolated from incubations of the adrenal with 11-deoxycortisol.

Author

Gomez-Sanchez CE, Foecking MF, Shackleton CH, Chavarri MR, and Gomez-Sanchez EP

Subjects

Animals, Cortodoxone analogs & derivatives, Cytochrome P-450 Enzyme System metabolism, Hydrocortisone metabolism, Male, Mass Spectrometry, Mixed Function Oxygenases metabolism, Rats, 17-Hydroxycorticosteroids metabolism, Adrenal Glands metabolism, Cortodoxone metabolism, Cytochrome P-450 CYP11B2

Abstract

Cortisol has been shown to be metabolized in the zona glomerulosa of the adrenal gland through the same pathway involving the cytochrome P-450, corticosterone methyl oxidase by which corticosterone is transformed to 18-hydroxycorticosterone and aldosterone. When cortisol is the precursor, 18-hydroxycortisol and 18-oxocortisol are formed. 18-Hydroxycortisol can also be made at a similar rate in the bovine zona fasciculata and reticularis as in the zona glomerulosa. We studied the possibility that the formation of 18-hydroxycortisol in the zona fasciculata and reticularis might be through a different pathway involving initial 18-hydroxylation of 11-deoxycortisol before 11 beta-hydroxylation. Rat adrenal capsules or cores were incubated with 10 micrograms of cortisol or 11-deoxycortisol and the formation of 18-hydroxycortisol was measured by radioimmunoassay. Both capsules and cores transformed 11-deoxycortisol to 18-hydroxycortisol, but cortisol was only transformed in the capsular portion. Sixty-two rat adrenals were incubated with 10 mg of 11-deoxycortisol and the putative steroid, 18-hydroxy-11-deoxycortisol, was purified by TLC and HPLC and subjected to gas chromatography mass spectrometry. The mass spectra indicated that the steroid isolated was indeed 18-hydroxy-11-deoxycortisol. The function of this steroid is still unknown.

Published

1987