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2. 21st century molecular biology in urology

Author

M, Williamson, S, Naaby-Hansen, and J R, Masters

Subjects
Genome, Proteome, Genetic Linkage, Drug Design, Urology, Mutation, Gene Expression, Humans, Nucleic Acid Hybridization, Molecular Biology, Neoplasm Proteins, Oligonucleotide Array Sequence Analysis
Published
2001

4. Differential extraction and enrichment of human sperm surface proteins in a proteome: identification of immunocontraceptive candidates

Author

J, Shetty, A B, Diekman, F C, Jayes, N E, Sherman, S, Naaby-Hansen, C J, Flickinger, and J C, Herr

Subjects
Adult, Male, Proteome, Octoxynol, Blotting, Western, Detergents, Molecular Sequence Data, Biotin, Succinimides, Buffers, Chemical Fractionation, Autoantigens, Polyethylene Glycols, Sequence Analysis, Protein, Humans, Urea, Biotinylation, Electrophoresis, Gel, Two-Dimensional, Amino Acid Sequence, Contraception, Immunologic, Infertility, Male, Autoantibodies, Saline Solution, Hypertonic, Membrane Proteins, Proteins, Spermatozoa, Cytoskeletal Proteins, Solubility, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Subtraction Technique, Solvents, Isoelectric Focusing, Acrosome
Abstract

The objective of this study was to discover previously unknown human sperm surface proteins that may be candidate contraceptive vaccinogens. To this end, methods of concentrating human sperm proteins for microsequencing by mass spectrometry were used, which increased the likelihood of identifying surface proteins. Vectorial labeling, differential extraction and two-dimensional (2-D) gel electrophoresis were employed to identify and isolate proteins accessible at the cell surface. Percoll harvested or swim-up sperm were either solubilized directly or solubilized after surface labeling with sulfo-succinimidyl-6-(biotinamido)hexanoate (sulfo-NHS-LC-biotin). Comparisons were made of proteins extracted with four lysis buffers: (i) Celis buffer containing 9.8 M urea and 2% Igepal CA-630; (ii) 1% Triton X (TX)-100; (iii) 1.7% TX-114 followed by phase partitioning; or (iv) 1 M NaCl. Blots of proteins separated by high-resolution 2-D electrophoresis were probed with avidin and antibodies to known proteins specific for three domains: the sperm surface (SAGA-1), the acrosome (SP-10), and the cytoskeleton (alpha-tubulin). Celis buffer (45 min) extracted proteins from all three major compartments. However, a 20-s extraction in Celis buffer enriched for several proteins and enabled the identification of several novel peptides by mass spectrometry. Mild extraction with TX-100 or 1 M NaCl solubilized mainly membrane and acrosomal proteins, but not cytoskeletal proteins. Comparison of biotinylated proteins extracted by each method showed that the major vectorially labeled proteins solubilized by Celis buffer were also solubilized by TX-100, TX-114, and 1 M NaCl. Extraction with TX-114 followed by phase-partitioning significantly enriched hydrophobic surface proteins and aided resolution and isolation. Eight protein spots microsequenced following all these extraction methods proved to be novel sperm molecules.

Published
2001

5. Differential nuclear localization of the cancer/testis-associated protein, SPAN-X/CTp11, in transfected cells and in 50% of human spermatozoa

Author

V A, Westbrook, A B, Diekman, S, Naaby-Hansen, S A, Coonrod, K L, Klotz, T S, Thomas, E J, Norton, C J, Flickinger, and J C, Herr

Subjects
Cell Nucleus, Male, Cytoplasm, X Chromosome, Nuclear Envelope, Blotting, Western, Molecular Sequence Data, Nuclear Proteins, Transfection, Spermatozoa, Cell Line, Molecular Weight, Solubility, Y Chromosome, Vacuoles, Animals, Humans, Amino Acid Sequence, Isoelectric Point, Fluorescent Antibody Technique, Indirect
Abstract

Cancer-testis antigens (CTAs) represent potential targets for cancer immunotherapy because these proteins are widely distributed in tumors but not in normal tissues, except testes. In this paper, we identify homology of the CTA CTp11 with SPAN-X (sperm protein associated with the nucleus mapped to the X chromosome). On two-dimensional Western blots of human sperm extracts, SPAN-X antibodies recognized 19 spots ranging from 20 to 23 kDa with isoelectric points from 5.0 to 5.5. Differential extraction of spermatozoa demonstrated that the SPAN-X protein is highly insoluble. Only 50% of ejaculated spermatozoa exhibited SPAN-X immunofluorescent staining. Dual localization of the sex chromosomes and the SPAN-X protein demonstrated that an equal number of X- and Y-bearing spermatozoa exhibited SPAN-X staining. In transfected mammalian CV1 cells, the SPAN-Xa and SPAN-Xb proteins were localized to the nucleus and cytoplasm, respectively, by indirect immunofluorescence. On immunoblots of CV1 cells, the SPAN-Xa protein migrated at 15-20 kDa, whereas the SPAN-Xb protein migrated at a higher molecular weight of 21-22 kDa. The SPAN-X protein was ultrastructurally associated with nuclear vacuoles and the redundant nuclear envelope. SPAN-X is the first protein specifically localized to these poorly characterized structures of the mammalian sperm nucleus and provides a unique biochemical marker for investigation of their function in spermatozoa as well as the role of SPAN-X/CTp11 in human tumors.

Published
2001

6. Anti-sperm antibodies from infertile patients and their cognate sperm antigens: a review. Identity between SAGA-1, the H6-3C4 antigen, and CD52

Author

Kenneth L. Klotz, John C. Herr, Elizabeth J. Norton, V A Westbrook, S Naaby-Hansen, and Alan B. Diekman

Subjects
Male, CD52, medicine.drug_class, Immunology, Monoclonal antibody, Isoantibodies, Antigen, Antigens, CD, Antigens, Neoplasm, medicine, Immunology and Allergy, Animals, Humans, Infertility, Male, Autoantibodies, Glycoproteins, biology, Obstetrics and Gynecology, Sperm Agglutination, Sperm, Spermatozoa, Reproductive Medicine, CD52 Antigen, Polyclonal antibodies, Antigens, Surface, biology.protein, Female, Antibody, Infertility, Female
Abstract

PROBLEM: The correlation of anti-sperm antibodies (ASA) with some instances of unexplained infertility implicates a role for these antibodies in blocking fertilization. Improved diagnosis and treatment of immunologic infertility, as well as a more complete understanding of the mechanism behind this phenomenon, are dependent on the identification and characterization of relevant sperm antigens. METHOD OF STUDY: In this article, we review literature on methods employed to identify sperm antigens using anti-sperm polyclonal and monoclonal antibodies from infertile patients and vasectomized men. Particular focus is given to approaches using human and mouse monoclonal antibodies to define the SAGA-1 human sperm antigen. RESULTS: ASA present in sera and genital tract secretions from infertile patients and vasectomized men have been employed in a variety of methods to identify sperm antigens. In an alternate approach, a monoclonal antibody (mAb), H6-3C4, was immortalized from the lymphocytes of an infertile woman who exhibited sperm-immobilizing titers. Subsequently, the sperm-agglutinating, murine S19 mAb was shown to react with the H6-3C4 cognate antigen. The H6-3C4/S19 cognate antigen, designated Sperm Agglutination Antigen-1 (SAGA-1), was characterized as a polymorphic, highly acidic, GPI-anchored glycoprotein on the surface of human spermatozoa. Purification with the S19 mAb followed by microsequencing demonstrated that the SAGA-1 core peptide is identical to CD52, a glycoprotein on the surface of human lymphocytes. Immunoblot analysis demonstrated that these two glycoproteins differed in carbohydrate composition. Thus, sperm SAGA-1 and lymphocyte CD52 represent glycoforms, glycoproteins with the same core peptide but with different carbohydrate structures. CONCLUSIONS: Autoimmunity to the SAGA-1 and/or CD52 glycoforms may lead to infertility. Structural and immunologic differences between these glycoproteins may be important factors in the etiology of immunologic infertility and other autoimmune disorders.

Published
2000

7. FSP95, a testis-specific 95-kilodalton fibrous sheath antigen that undergoes tyrosine phosphorylation in capacitated human spermatozoa

Author

A, Mandal, S, Naaby-Hansen, M J, Wolkowicz, K, Klotz, J, Shetty, J D, Retief, S A, Coonrod, M, Kinter, N, Sherman, F, Cesar, C J, Flickinger, and J C, Herr

Subjects
Male, DNA, Complementary, Molecular Sequence Data, Proteins, In Vitro Techniques, Blotting, Northern, Spermatozoa, Recombinant Proteins, Molecular Weight, Blotting, Southern, Infertility, Testis, Escherichia coli, Humans, Tyrosine, Amino Acid Sequence, Cloning, Molecular, Phosphorylation, Sperm Capacitation
Abstract

Protein tyrosine phosphorylation has been associated with both capacitation and motility of mammalian sperm. During capacitation, human spermatozoa undergo tyrosine phosphorylation of a characteristic set of proteins, only one of which has thus far been cloned and localized. We report here the sequence of a fibrous sheath protein of 95 kDa (FSP95) that undergoes tyrosine phosphorylation during capacitation of human spermatozoa and has similarity to sperm A-kinase anchor proteins (AKAPs). FSP95 is both auto- and iso-antigenic in humans as it is recognized by sera containing antisperm antibodies from infertile men and women. The 853-residue protein has a calculated molecular weight of 94.6 kDa and an isoelectric point (pI) of 6.0, and it contains multiple potential phosphorylation sites for protein kinase C and casein kinase II as well as one potential tyrosine kinase phosphorylation site at amino acid 435. The sequence has amino acid homology to mouse sperm fibrous sheath AKAP82 (pro-mAKAP82, 34% identity) and to human sperm fibrous sheath AKAP82 (pro-hAKAP82, 32% identity). The gene encoding FSP95 has 5 exons separated by 4 introns and is located on chromosome 12 at locus p13.3. Northern analysis detected a single transcript of approximately 3.0 kilobases, and Northern dot blot analysis of 50 human tissues revealed FSP95 mRNA expression only in testis. By employing sperm immobilization, indirect immunofluorescence, and immunoelectron microscopy with antisera to purified recombinant FSP95, the protein was localized to the ribs of the fibrous sheath in the principal piece of the sperm tail. FSP95 is the second fibrous sheath protein to be cloned, sequenced and localized in human spermatozoa.

Published
1999

8. Human sperm proteome: immunodominant sperm surface antigens identified with sera from infertile men and women

Author

J, Shetty, S, Naaby-Hansen, H, Shibahara, R, Bronson, C J, Flickinger, and J C, Herr

Subjects
Male, Sex Characteristics, Immune Sera, Blotting, Western, Proteins, Hydrogen-Ion Concentration, Spermatozoa, Immunoglobulin M, Immunoglobulin G, Antigens, Surface, Luminescent Measurements, Humans, Electrophoresis, Polyacrylamide Gel, Female, Isoelectric Focusing, Infertility, Female, Infertility, Male
Abstract

The objective of this study was to identify those immunodominant sperm antigens recognized by antisperm antibodies (ASA) in the serum samples of infertile men and women. High-resolution two-dimensional gel electrophoresis was employed to separate human sperm proteins using isoelectric focusing or nonequilibrium pH gradient electrophoresis, followed by PAGE. Serum samples from 15 infertile male subjects and 6 infertile female subjects that contained ASA as assayed by the immunobead binding test (IBT) were analyzed by Western blotting followed by enhanced chemiluminescence (ECL). Serum samples from 10 fertile subjects (5 males and 5 females) that were ASA negative by IBT were used as controls. The ECL blots were analyzed by computer scanning to compare the immunoreactivity between serum samples from fertile and infertile subjects and to identify the antigens unique to the sera of the infertile subjects; 98 sperm auto- and iso-antigenic protein spots were recognized by sera from infertile males and females but not from fertile subjects. Based on vectorial labeling with 125I at the sperm surface, a subset of 6 auto- and iso-antigens was identified as possibly relevant to antibody-mediated infertility.

Published
1999

9. Biochemical characterization of sperm agglutination antigen-1, a human sperm surface antigen implicated in gamete interactions

Author

A B, Diekman, V A, Westbrook-Case, S, Naaby-Hansen, K L, Klotz, C J, Flickinger, and J C, Herr

Subjects
Male, Membrane Glycoproteins, Detergents, Immunoblotting, Periodic Acid, Antibodies, Monoclonal, In Vitro Techniques, Sperm Agglutination, Spermatozoa, Microscopy, Fluorescence, Fluorescent Antibody Technique, Direct, Semen, Antigens, Surface, Humans, Electrophoresis, Polyacrylamide Gel
Abstract

The anti-sperm monoclonal antibody (mAb) S19 was previously demonstrated to agglutinate human spermatozoa, inhibit sperm penetration of cervical mucus, and inhibit sperm-zona pellucida binding. These results implicated the cognate S19 antigen, designated sperm agglutination antigen-1 (SAGA-1), in gamete interactions and identified SAGA-1 as an attractive candidate for immunocontraceptive development. In the present study, evaluation of sperm agglutination with video microscopy showed that the S19 mAb rapidly and completely agglutinated human spermatozoa in a "tangled" pattern of agglutination. One- and two-dimensional immunoblot analyses identified SAGA-1 as a highly acidic, polymorphic sperm protein with an apparent molecular mass of 15-25 kDa and an isoelectric point of 2.5-3.0. Periodate treatment abolished this immunoreactivity, demonstrating that the S19 mAb reacted with a carbohydrate epitope and indicating that SAGA-1 is a glycoprotein. Absence of S19 immunoreactivity in postvasectomy seminal fluid implicated the testis, epididymis, and/or proximal vas deferens in the expression of SAGA-1. In solubility and phase partitioning assays, SAGA-1 was extracted from spermatozoa in Triton X-114 and exhibited the hydrophobic characteristics of integral and glycosylphosphatidyl inositol-anchored membrane proteins. These results identify SAGA-1 as a hydrophobic, highly acidic sperm glycoprotein that is localized on the entire sperm surface and has potential significance as a target for antibodies that inhibit sperm function and gamete interactions.

Published
1997

10. Two-dimensional gel electrophoretic analysis of vectorially labeled surface proteins of human spermatozoa

Author

S, Naaby-Hansen, C J, Flickinger, and J C, Herr

Subjects
Male, Silver Staining, Immunoblotting, Biotin, Membrane Proteins, Blood Proteins, Spermatozoa, Iodine Radioisotopes, Solubility, Semen, Image Processing, Computer-Assisted, Humans, Electrophoresis, Polyacrylamide Gel, Isoelectric Focusing
Abstract

The objective of this study was to identify the repertoire of proteins exposed on the surface of ejaculated human spermatozoa. High-resolution two-dimensional gel systems for separation of human sperm and seminal plasma proteins were developed using both isoelectric focusing (IEF) and nonequilibrium pH gradient electrophoresis (NEPHGE) followed by polyacrylamide gel electrophoresis (IEF/PAGE, NEPHGE/PAGE). Proteins were visualized by silver staining of gels and by electroblotting followed by gold staining. The protein patterns were analyzed by computer after laser or camera scanning. One thousand three hundred ninety-seven sperm proteins with a molecular mass between 5 and 160 kDa and isoelectric points (pI) from 4 to 11 were catalogued from silver-stained gels loaded with approximately 0.25 mg of NP-40/urea extracts of sperm harvested by Percoll density gradient centrifugation, and 1191 proteins were resolved following extraction with SDS/3-[3-cholamidopropyl) dimethylammonio]-1-propane-sulfonate/urea. Analysis of seminal plasma proteins obtained from vasectomized patients revealed over 300 silver-stained proteins, which aided the identification of sperm-coating proteins acquired from secretions of the accessory sex organs. Sperm surface proteins accessible to vectorial labeling with 125I or N-hydroxysuccinimide biotin were identified; 181 protein spots were radiolabeled with 125I, while 228 protein spots were biotinylated, including several groups of protein isoforms. Cytoskeletal and intra-acrosomal control proteins were not iodinated or biotinylated, thus verifying the surface specificity of both labeling methods. Ninety-eight sperm surface proteins were labeled by both iodine and biotin, and 22 sperm surface proteins, representing five groups of protein isoforms, were shown to contain phosphotyrosine. A composite computer image showing the position of the dually vectorially labeled sperm surface proteins was constructed, together with a table of the proteins' molecular weight, pI, and relative concentration. In addition, novel isoforms of actin, beta-tubulin, PH-20, and several phosphotyrosine-containing proteins were identified in human sperm.

Published
1997

11. Complementary deoxyribonucleic acid cloning and characterization of mSP-10: the mouse homologue of human acrosomal protein SP-10

Author

P P, Reddi, S, Naaby-Hansen, I, Aguolnik, J Y, Tsai, L M, Silver, C J, Flickinger, and J C, Herr

Subjects
DNA, Complementary, Base Sequence, Immunoblotting, Molecular Sequence Data, Chromosome Mapping, Membrane Proteins, Sequence Homology, Recombinant Proteins, Mice, Escherichia coli, Animals, Humans, Electrophoresis, Gel, Two-Dimensional, Amino Acid Sequence, Antigens, Cloning, Molecular, Gonadal Steroid Hormones, Acrosome, Sequence Analysis, Polymorphism, Restriction Fragment Length
Abstract

Complementary DNA encoding the putative mouse homologue for human acrosomal protein SP-10, a candidate contraceptive vaccinogen, was cloned and sequenced. The entire open reading frame (amino acids 18 to 261) of the mouse SP-10 (mSP-10), with the exception of the signal peptide (amino acids 1 to 17), was placed under the influence of inducible T7 RNA polymerase/promoter system to overproduce recombinant protein (re-mSP-10) in Escherichia coli. A six-histidine tag, which was coexpressed at the carboxyl terminus of re-mSP-10, provided the means for purification of re-mSP-10 by immobilized metal chelation affinity chromatography technique. The level of purity of re-mSP-10 thus obtained was determined by 2-dimensional gel electrophoresis to be 98%. Immunoblotting with monoclonal and polyclonal antibodies previously generated against human or baboon SP-10 showed that mSP-10 shared significant antigenic similarity with its primate counterparts. The position of mSP-10 in the mouse genome was next mapped through segregation analysis of an interspecific backcross panel of 96 animals. Acrv1 (assigned gene symbol for mSP-10) was localized in the proximal portion of mouse chromosome 9 in a region that exhibits synteny with human 11q23, the region to which ACRV1 (gene symbol for human SP-10) was previously mapped. These characterizations by combined immunological and gene mapping techniques established the cloned mSP-10 to be the mouse homologue of SP-10.

Published
1995

12. The potential role of IL-1 in the ovulatory process: an evolving hypothesis

Author

I. A. Lea, Eli Y. Adashi, C. Weston, C. J. Flickinger, S. Naaby-Hansen, R. Bhattacharya, J. C. Herr, Michael G. O'Rand, B. E. Kurth, K. S.K. Tung, F. Foley, D. Bryant, and Prabhakara Poothi Reddi

Subjects
Immunocontraception, medicine.anatomical_structure, Reproductive Medicine, Immunology, medicine, Obstetrics and Gynecology, Immunology and Allergy, Gamete, Biology
Published
1997
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15. Functional proteomic analysis of long-term growth factor stimulation and receptor tyrosine kinase coactivation in Swiss 3T3 fibroblasts.

Author

Nagano K, Akpan A, Warnasuriya G, Corless S, Totty N, Yang A, Stein R, Zvelebil M, Stensballe A, Burlingame A, Waterfield M, Cramer R, Timms JF, and Naaby-Hansen S

Subjects
3T3 Cells, Animals, Benzamides pharmacology, Calcium-Calmodulin-Dependent Protein Kinases antagonists & inhibitors, Cell Line, Chromones pharmacology, Enzyme Inhibitors pharmacology, Fibroblasts, Flavonoids pharmacology, Isotope Labeling, Mice, Morpholines pharmacology, Nucleosome Assembly Protein 1 metabolism, Phosphoinositide-3 Kinase Inhibitors, Phosphorylation drug effects, Proto-Oncogene Proteins c-akt metabolism, Receptor Protein-Tyrosine Kinases metabolism, Receptors, Platelet-Derived Growth Factor metabolism, Signal Transduction drug effects, Epidermal Growth Factor pharmacology, Insulin-Like Growth Factor I pharmacology, Phosphatidylinositol 3-Kinases metabolism, Platelet-Derived Growth Factor pharmacology, Proteome analysis
Abstract

In Swiss 3T3 fibroblasts, long-term stimulation with PDGF, but not insulin-like growth factor 1 (IGF-1) or EGF, results in the establishment of an elongated migratory phenotype, characterized by the formation of retractile dendritic protrusions and absence of actin stress fibers and focal adhesion complexes. To identify receptor tyrosine kinase-specific reorganization of the Swiss 3T3 proteome during phenotypic differentiation, we compared changes in the pattern of protein synthesis and phosphorylation during long-term exposure to PDGF, IGF-1, EGF, and their combinations using 2DE-based proteomics after (35)S- and (33)P-metabolic labeling. One hundred and five differentially regulated proteins were identified by mass spectrometry and some of these extensively validated. PDGF stimulation produced the highest overall rate of protein synthesis at any given time and induced the most sustained phospho-signaling. Simultaneous activation with two or three of the growth factors revealed both synergistic and antagonistic effects on protein synthesis and expression levels with PDGF showing dominance over both IGF-1 and EGF in generating distinct proteome compositions. Using signaling pathway inhibitors, PI3K was identified as an early site for signal diversification, with sustained activity of the PI3K/AKT pathway critical for regulating late protein synthesis and phosphorylation of target proteins and required for maintaining the PDGF-dependent motile phenotype. Several proteins were identified with novel PI3K/Akt-dependent synthesis and phosphorylations including eEF2, PRS7, RACK-1, acidic calponin, NAP1L1, Hsp73, and fascin. The data also reveal induction/suppression of key F-actin and actomyosin regulators and chaperonins that enable PDGFR to direct the assembly of a motile cytoskeleton, despite simultaneous antagonistic signaling activities. Together, the study demonstrates that long-term exposure to different growth factors results in receptor tyrosine kinase-specific regulation of relatively small subproteomes, and implies that the strength and longevity of receptor tyrosine kinase-specific signals are critical in defining the composition and functional activity of the resulting proteome.

Published
2012
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16. Functional and immunological analysis of the human sperm proteome.

Author

Naaby-Hansen S

Subjects
Antibodies immunology, Autoimmunity genetics, Autoimmunity immunology, Databases, Factual, Electrophoresis, Gel, Pulsed-Field, Glycosylphosphatidylinositols immunology, Humans, Male, Proteome genetics, Spermatogenesis genetics, Proteome immunology, Spermatozoa immunology
Abstract

This is a review of ten previously published studies of the human sperm proteome. Proteins expressed on the sperm cell surface were identified and characterized by a combination of vectorial labelling with radioiodine and biotin, PI-PLC treatment, two-dimensional gel electrophoresis, immuno and lectin blotting procedures, affinity overlay assays with radioactive nucleotide triphosphates and 45Ca, and mass spectrometry analysis. Examination of capacitation-induced modifications of the human sperm proteome led to the cloning and characterisation of two new phospho-regulated cancer-testis antigens, which we named Fibrous Sheath Protein 95 (FSP95) and CABYR (calcium-binding tyrosine phosphorylation regulated). A protein kinase A RII binding domain is present between amino acids 124 and 141 identifying FSP95 (now commonly known as AKAP3) as a member of the A kinase anchoring protein-family which provides spatial and temporal specificity to the cAMP-PKA pathway. In addition to scaffolding PKA, PDE and protein phosphatases, AKAPs also bind to a group of four proteins that share homology to the RII dimerization/docking (R2D2) domain of PKA' regulatory subunit. CABYR, which is one of these four proteins, also interacts with a diverse array of signal tranducers via its SH3-, R2D2-, and proline-rich extension-like domains. AKAP3 and CABYR appear to associate in high molecular weight multi-protein complexes, which regulate the flagella' energy supply and movements. Diagonal gel electrophoresis experiments suggest that the high molecular weight signal-integrating scaffold partly is established by homo- and hetero-oligomerization of lower molecular weight splice variants of CABYR. The putative role of CABYR in lung cancer cells is finally discussed.

Published
2012

17. Identification of calcium-binding proteins associated with the human sperm plasma membrane.

Author

Naaby-Hansen S, Diekman A, Shetty J, Flickinger CJ, Westbrook A, and Herr JC

Subjects
Calcium metabolism, Calcium-Binding Proteins chemistry, Calcium-Binding Proteins metabolism, Electrophoresis, Gel, Two-Dimensional, Endoplasmic Reticulum Chaperone BiP, Humans, Male, Semen Analysis methods, Sperm Agglutination physiology, Sperm Capacitation physiology, Young Adult, Calcium-Binding Proteins isolation & purification, Cell Membrane metabolism, Spermatozoa metabolism
Abstract

Background: The precise composition of the human sperm plasma membrane, the molecular interactions that define domain specific functions, and the regulation of membrane associated proteins during the capacitation process, still remain to be fully understood. Here, we investigated the repertoire of calcium-regulated proteins associated with the human sperm plasma membrane., Methods: Surface specific radioiodination was combined with two-dimensional gel electrophoresis, a 45Ca-overlay assay, computer assisted image analysis and mass spectrometry to identify calcium-binding proteins exposed on the human sperm surface., Results: Nine acidic 45Ca-binding sperm proteins were excised from stained preparative 2D gels and identified by mass spectrometry. Five of the calcium binding proteins; HSPA2 (HSP70-1), HSPA5 (Bip), HYOU1 (ORP150), serum amyloid P-component (SAP) and protein kinase C substrate 80K-H (80K-H) were found to be accessible to Iodo-Bead catalyzed 125I-labelling on the surface of intact human sperm. Agglutination and immunofluorescence analysis confirmed that SAP is situated on the plasma membrane of intact, motile sperm as well as permeabilized cells. Western blot analysis showed increased phosphorylation of human sperm 80K-H protein following in vitro capacitation. This is the first demonstration of the 80K-H protein in a mammalian sperm., Conclusion: The presence of SAP on the surface of mature sperm implies that SAP has a physiological role in reproduction, which is thought to be in the removal of spermatozoa from the female genital tract via phagocytosis. Since 80K-H is a Ca2+-sensor recently implicated in the regulation of both inositol 1,4,5-trisphosphate receptor and transient receptor potential (TRP) cation channel activities, its detection in sperm represents the first direct signaling link between PKC and store-operated calcium channels identified in human sperm.

Published
2010
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18. Heat shock proteins on the human sperm surface.

Author

Naaby-Hansen S and Herr JC

Subjects
Acrosome Reaction immunology, Animals, Antigens immunology, Chlamydia Infections immunology, Endoplasmic Reticulum Chaperone BiP, Epitopes immunology, Female, Heat-Shock Proteins chemistry, Humans, Male, Molecular Chaperones chemistry, Molecular Chaperones metabolism, Rabbits, Spermatozoa chemistry, Cell Membrane metabolism, Heat-Shock Proteins metabolism, Spermatozoa metabolism
Abstract

The sperm plasma membrane is known to be critical to fertilization and to be highly regionalized into domains of head, mid- and principal pieces. However, the molecular composition of the sperm plasma membrane and its alterations during genital tract passage, capacitation and the acrosome reaction remains to be fully dissected. A two-dimensional gel-based proteomic study previously identified 98 human sperm proteins which were accessible for surface labelling with both biotin and radioiodine. In this report twelve dually labelled protein spots were excised from stained gels or PDVF membranes and analysed by mass spectrometry (MS) and Edman degradation. Seven members from four different heat shock protein (HSP) families were identified including HYOU1 (ORP150), HSPC1 (HSP86), HSPA5 (Bip), HSPD1 (HSP60), and several isoforms of the two testis-specific HSP70 chaperones HSPA2 and HSPA1L. An antiserum raised against the testis-specific HSPA2 chaperone reacted with three 65kDa HSPA2 isoforms and three high molecular weight surface proteins (78-79kDa, 84kDa and 90-93kDa). These proteins, together with seven 65kDa HSP70 forms, reacted with human anti-sperm IgG antibodies that blocked in vitro fertilization in humans. Three of these surface biotinylated human sperm antigens were immunoprecipitated with a rabbit antiserum raised against a linear peptide epitope in Chlamydia trachomatis HSP70. The results indicate diverse HSP chaperones are accessible for surface labelling on human sperm. Some of these share epitopes with C. trachomatis HSP70, suggesting an association between genital tract infection, immunity to HSP70 and reproductive failure., (2009 Elsevier Ireland Ltd. All rights reserved.)

Published
2010
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19. Interferon-gamma reduces cell surface expression of annexin 2 and suppresses the invasive capacity of prostate cancer cells.

Author

Hastie C, Masters JR, Moss SE, and Naaby-Hansen S

Subjects
Cell Line, Tumor, Epithelial Cells drug effects, Epithelial Cells enzymology, Epithelial Cells pathology, Humans, Hydrolases metabolism, Male, Neoplasm Invasiveness, Protein Transport drug effects, Annexins metabolism, Cell Membrane metabolism, Interferon-gamma pharmacology, Prostatic Neoplasms metabolism, Prostatic Neoplasms pathology
Abstract

The effect of interferon-gamma (IFNgamma) treatment on cell surface protein expression was studied in the human prostate cancer cell line 1542CP3TX. IFNgamma increased both the number and abundance of proteins in membrane fractions. In contrast, the expression of annexin 2 and its binding partner p11 decreased by 4-fold after 24 h of exposure, with the remaining anx2(t) complexes localized to lipid rafts. Within the same time scale, IFNgamma reduced the abundance of the peripherally attached, anx2(t)-associated proteases procathepsin B and plasminogen. The invasive capacity of the cancer cells was reduced by treatment with IFNgamma or antibody to annexin 2 in 1542CP3TX cells, but not in LNCaP, an annexin 2-negative prostate cancer cell line. Expression of annexin 2 in LNCaP cells increased their invasiveness. IFNgamma induced calpain expression and activation and increased the phosphorylation and degradation of the calpain substrate ABCA1 in 1542CP3TX cancer cells. Surface expression of annexin 2 was reduced in cells treated with glyburide, an ABCA1 inhibitor, whereas inhibition of calpain abrogated IFNgamma-induced annexin 2 down-regulation and suppression of Matrigel invasion. The findings suggest annexin 2 externalization is coupled to lipid efflux in prostate epithelium and that IFNgamma induces down-regulation of the protease-binding anx2(t) scaffold at the cell surface and consequently acts to suppress invasiveness through calpain-mediated degradation of the lipid transporter ABCA1.

Published
2008
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20. Gene and protein expression profiling of human ovarian cancer cells treated with the heat shock protein 90 inhibitor 17-allylamino-17-demethoxygeldanamycin.

Author

Maloney A, Clarke PA, Naaby-Hansen S, Stein R, Koopman JO, Akpan A, Yang A, Zvelebil M, Cramer R, Stimson L, Aherne W, Banerji U, Judson I, Sharp S, Powers M, deBilly E, Salmons J, Walton M, Burlingame A, Waterfield M, and Workman P

Subjects
Acetylation, Biopsy, Cell Line, Tumor, Female, Gene Expression Profiling, HCT116 Cells, HSP90 Heat-Shock Proteins biosynthesis, Humans, Macrolides pharmacology, Neoplasm Proteins biosynthesis, Neoplasm Proteins genetics, Neoplasm Proteins metabolism, Ovarian Neoplasms genetics, Ovarian Neoplasms metabolism, Ovarian Neoplasms pathology, Protein Methyltransferases metabolism, Protein-Arginine N-Methyltransferases, Proteomics, Benzoquinones pharmacology, HSP90 Heat-Shock Proteins antagonists & inhibitors, Lactams, Macrocyclic pharmacology, Ovarian Neoplasms drug therapy
Abstract

The promising antitumor activity of 17-allylamino-17-demethoxygeldanamycin (17AAG) results from inhibition of the molecular chaperone heat shock protein 90 (HSP90) and subsequent degradation of multiple oncogenic client proteins. Gene expression microarray and proteomic analysis were used to profile molecular changes in the A2780 human ovarian cancer cell line treated with 17AAG. Comparison of results with an inactive analogue and an alternative HSP90 inhibitor radicicol indicated that increased expression of HSP72, HSC70, HSP27, HSP47, and HSP90beta at the mRNA level were on-target effects of 17AAG. HSP27 protein levels were increased in tumor biopsies following treatment of patients with 17AAG. A group of MYC-regulated mRNAs was decreased by 17AAG. Of particular interest and novelty were changes in expression of chromatin-associated proteins. Expression of the heterochromatin protein 1 was increased, and expression of the histone acetyltransferase 1 and the histone arginine methyltransferase PRMT5 was decreased by 17AAG. PRMT5 was shown to be a novel HSP90-binding partner and potential client protein. Cellular protein acetylation was reduced by 17AAG, which was shown to have an antagonistic interaction on cell proliferation with the histone deacetylase inhibitor trichostatin A. This mRNA and protein expression analysis has provided new insights into the complex molecular pharmacology of 17AAG and suggested new genes and proteins that may be involved in response to the drug or be potential biomarkers of drug action.

Published
2007
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21. PDGF regulates the actin cytoskeleton through hnRNP-K-mediated activation of the ubiquitin E3-ligase MIR.

Author

Nagano K, Bornhauser BC, Warnasuriya G, Entwistle A, Cramer R, Lindholm D, and Naaby-Hansen S

Subjects
Actin Cytoskeleton drug effects, Actin Cytoskeleton metabolism, Actins metabolism, Animals, Cell Movement, Cytoskeleton metabolism, Cytoskeleton ultrastructure, Down-Regulation, Enzyme Activation, Epidermal Growth Factor pharmacology, Fibroblasts drug effects, Fibroblasts physiology, Fibroblasts ultrastructure, Insulin-Like Growth Factor I pharmacology, Mice, Myosin Light Chains metabolism, Proteasome Endopeptidase Complex, Proteasome Inhibitors, RNA, Small Interfering genetics, RNA, Small Interfering pharmacology, Swiss 3T3 Cells, Ubiquitin-Protein Ligases antagonists & inhibitors, Ubiquitin-Protein Ligases genetics, src-Family Kinases antagonists & inhibitors, Actins drug effects, Cytoskeleton drug effects, Heterogeneous-Nuclear Ribonucleoprotein K metabolism, Platelet-Derived Growth Factor pharmacology, Ubiquitin-Protein Ligases metabolism
Abstract

PDGF is a potent chemotactic mitogen and a strong inductor of fibroblast motility. In Swiss 3T3 fibroblasts, exposure to PDGF but not EGF or IGF-1 causes a rapid loss of actin stress fibers (SFs) and focal adhesions (FAs), which is followed by the development of retractile dendritic protrusions and induction of motility. The PDGF-specific actin reorganization was blocked by inhibition of Src-kinase and the 26S proteasome. PDGF induced Src-dependent association between the multifunctional transcription/translation regulator hnRNP-K and the mRNA-encoding myosin regulatory light-chain (MRLC)-interacting protein (MIR), a E(3)-ubiquitin ligase that is MRLC specific. This in turn rapidly increased MIR expression, and led to ubiquitination and proteasome-mediated degradation of MRLC. Downregulation of MIR by RNA muting prevented the reorganization of actin structures and severely reduced the migratory and wound-healing potential of PDGF-treated cells. The results show that activation of MIR and the resulting removal of diphosphorylated MRLC are essential for PDGF to instigate and maintain control over the actin-myosin-based contractile system in Swiss 3T3 fibroblasts. The PDGF induced protein destabilization through the regulation of hnRNP-K controlled ubiquitin -ligase translation identifies a novel pathway by which external stimuli can regulate phenotypic development through rapid, organelle-specific changes in the activity and stability of cytoskeletal regulators.

Published
2006
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22. Translation and assembly of CABYR coding region B in fibrous sheath and restriction of calcium binding to coding region A.

Author

Kim YH, Jha KN, Mandal A, Vanage G, Farris E, Snow PL, Klotz K, Naaby-Hansen S, Flickinger CJ, and Herr JC

Subjects
Alternative Splicing, Animals, Antibodies, Base Sequence, Calcium metabolism, Calcium-Binding Proteins chemistry, Calcium-Binding Proteins immunology, Cloning, Molecular, Codon, Terminator, DNA, Complementary genetics, Humans, Male, Microscopy, Electron, Phosphoproteins chemistry, Phosphoproteins immunology, Polymorphism, Genetic, Protein Biosynthesis, Protein Isoforms chemistry, Protein Isoforms genetics, Protein Isoforms metabolism, Rats, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins immunology, Recombinant Proteins metabolism, Sperm Tail ultrastructure, Spermatogenesis, Calcium-Binding Proteins genetics, Calcium-Binding Proteins metabolism, Phosphoproteins genetics, Phosphoproteins metabolism, Sperm Tail metabolism
Abstract

CABYR is a highly polymorphic, sperm flagellar calcium-binding protein that is tyrosine as well as serine/threonine phosphorylated during capacitation. Six alternative splice variants of human CABYR (I-VI) have previously been identified, involving two coding regions, CR-A and CR-B, separated by an intervening stop codon. It is presently unknown if proteins encoded by the predicted coding region B of CABYR are translated during spermiogenesis, where they localize, or which CABYR isoforms bind calcium. Immunofluorescent and electron microscopic studies using polyclonal antibodies generated to the recombinant c-terminal 198 aa CABYR-B localized the isoforms containing CABYR-B to the ribs and longitudinal columns of the fibrous sheath in the principal piece of the flagellum. Antisera to recombinant CABYR-A and CABYR-B proteins recognized distinct populations of CABYR isoforms encoded by either CR-A alone and/or CR-B as well as a common population of CABYR isoforms. Only the recombinant CABYR-A and not the CABYR-B bound calcium in vitro, which is consistent with the hypothesis that CABYR-A is the only form that binds calcium in sperm. These observations confirmed that, despite the presence of the stop codon in CR-A, splice variants containing CR-B are expressed during spermiogenesis and assemble into the fibrous sheath of the principal piece; however, calcium binding occurs only to those CABYR isoforms containing CABYR-A.

Published
2005
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23. Combined affinity labelling and mass spectrometry analysis of differential cell surface protein expression in normal and prostate cancer cells.

Author

Hastie C, Saxton M, Akpan A, Cramer R, Masters JR, and Naaby-Hansen S

Subjects
Cell Line, Tumor, Cell Membrane drug effects, Electrophoresis, Gel, Two-Dimensional, Humans, Image Processing, Computer-Assisted, Immunoblotting, Interferons pharmacology, Male, Membrane Proteins drug effects, Cell Membrane metabolism, Chromatography, Affinity, Mass Spectrometry, Membrane Proteins metabolism, Prostatic Neoplasms metabolism
Abstract

Differences in the expression of cell surface proteins between a normal prostate epithelial (1542-NP2TX) and a prostate cancer cell line (1542-CP3TX) derived from the same patient were investigated. A combination of affinity chromatographic purification of biotin-tagged surface proteins with mass spectrometry analysis identified 26 integral membrane proteins and 14 peripheral surface proteins. The findings confirm earlier reports of altered expression in prostate cancer for several cell surface proteins, including ALCAM/CD166, the Ephrin type A receptor, EGFR and the prostaglandin F2 receptor regulatory protein. In addition, several novel findings of differential expression were made, including the voltage-dependent anion selective channel proteins Porin 1 and 2, ecto-5'-nucleotidase (CD73) and Scavenger receptor B1. Cell surface protein expression changed both qualitatively and quantitatively when the cells were grown in the presence of either or both interferon INFalpha and INFgamma. Costimulation with type I and II interferons had additive or synergistic effects on the membrane density of several, mainly peripherally attached surface proteins. Concerted upregulation of surface exposed antigens may be of benefit in immuno-adjuvant-based treatment of interferon-responsive prostate cancer. In conclusion, this study demonstrates that differences in the expression of membrane proteins between normal and prostate cancer cells are reproducibly detectable following vectorial labelling with biotin, and that detailed analysis of extracellular-induced surface changes can be achieved by combining surface-specific labelling with high-resolution two-dimensional gel electrophoresis and mass spectrometry.

Published
2005
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24. Proteomic approaches in the analysis of hypertension.

Author

Naaby-Hansen S, Warnasuriya GD, Hastie C, Gallney P, and Cramer R

Subjects
Amino Acid Sequence, Electrophoresis, Gel, Two-Dimensional, Humans, Mass Spectrometry, Molecular Sequence Data, Hypertension genetics, Proteome
Abstract

The completion of the genomic sequence and the definition of the genes provide a wealth of data to interpret cellular protein expression patterns and relate them to protein function. Proteomics is the large-scale study of proteins in the post-genomic era, aimed at identifying and characterizing protein expression, function, posttranslational modification, regulation, trafficking, interaction and structure, and their perturbation by disease and drug action. The multigenetic background and essentially unknown etiology of hypertension, makes this main killer a prime candidate for proteomic analysis. The classical proteomic approaches are based on two-dimensional gel electrophoretic protein separation and their subsequent identification and characterization by mass spectrometry analysis. However, expression level analysis may not reflect the functional state of proteins and is biased towards long-lived abundant proteins. This review describes a variety of techniques that can be used to identify low-abundance proteins that may be of more functional interest. The modification of classical two-dimensional electrophoresis in order to study post-translational modifications, e.g., phosphorylation, is also discussed.

Published
2005
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25. Differential protein synthesis and expression levels in normal and neoplastic human prostate cells and their regulation by type I and II interferons.

Author

Nagano K, Masters JR, Akpan A, Yang A, Corless S, Wood C, Hastie C, Zvelebil M, Cramer R, and Naaby-Hansen S

Subjects
Carrier Proteins metabolism, Cell Division drug effects, Cell Line, Cell Line, Tumor, DNA-Binding Proteins biosynthesis, Electrophoresis, Gel, Two-Dimensional, Epidermal Growth Factor pharmacology, GTP-Binding Proteins biosynthesis, Heterogeneous-Nuclear Ribonucleoprotein K biosynthesis, Humans, Interferon-Stimulated Gene Factor 3, Interferon-Stimulated Gene Factor 3, gamma Subunit, Male, Mitogen-Activated Protein Kinases metabolism, Myxovirus Resistance Proteins, Phosphatidylinositol 3-Kinases metabolism, Phosphorylation drug effects, Prostate cytology, Prostate pathology, Prostatic Neoplasms enzymology, Prostatic Neoplasms pathology, Signal Transduction drug effects, Spectrometry, Mass, Electrospray Ionization, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Transcription Factors biosynthesis, Gene Expression Profiling, Gene Expression Regulation, Neoplastic drug effects, Interferon-alpha pharmacology, Interferon-gamma pharmacology, Intracellular Signaling Peptides and Proteins, Prostate metabolism, Prostatic Neoplasms metabolism, Proteome biosynthesis
Abstract

Protein expression and de novo synthesis in normal and prostate cancer cell lines derived from the same patient were compared by proteomic analysis, and the effects of INFalpha and INFgamma (INF=interferon) determined. The expressions of several INF-inducible proteins, including MxA, Nmi, PA28a and IFP53, were downregulated in the cancer cells. INFgamma induced a more than twofold increase or decrease in the synthesis rates of almost twice as many proteins in the cancer cell line. The positive regulator of INF-induced transcription ISGF3gamma was upregulated in the cancer cells and inversely regulated by INFalpha and INFgamma in the normal and cancer cells. Moreover, ISGF3gamma's induction by INFgamma in the cancer cells was more enhanced by simultaneous stimulation with EGF, than its induction in the normal cells. In all, 31 differentially regulated proteins were identified by mass spectrometry analysis, several of which are involved in chaperone-assisted protein folding in the endoplasmic reticulum (ER) or in regulated protein degradation. Our results suggest that the exclusion of proteins by the ER quality control system, crosstalk between the EGF- and INF-induced signalling pathways and the regulation of INF-inducible genes are all altered in the prostate cancer cells. The combination of upregulated activity in the growth-promoting PI3K/Akt pathway, suppression of Nmi and overexpression of hnRNP-K and c-myc proteins may explain why the prostate cancer cells were found to be more resistant to the growth inhibitory effects of INFgamma.

Published
2004
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26. Proteomics in the analysis of prostate cancer.

Author

Naaby-Hansen S, Nagano K, Gaffney P, Masters JR, and Cramer R

Subjects
Electrophoresis, Gel, Two-Dimensional methods, Gene Expression Profiling, Gene Expression Regulation, Neoplastic, Humans, Male, RNA, Messenger analysis, Signal Transduction, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods, Antigens, Neoplasm analysis, Biomarkers, Tumor analysis, Neoplasm Proteins analysis, Prostatic Neoplasms chemistry, Proteomics
Published
2003
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27. Activation of the ATPase activity of hsp90 by the stress-regulated cochaperone aha1.

Author

Panaretou B, Siligardi G, Meyer P, Maloney A, Sullivan JK, Singh S, Millson SH, Clarke PA, Naaby-Hansen S, Stein R, Cramer R, Mollapour M, Workman P, Piper PW, Pearl LH, and Prodromou C

Subjects
Cell Line, Transformed, Centromere genetics, Circular Dichroism, Cloning, Molecular, Genes, src, Genetic Vectors, HSP90 Heat-Shock Proteins genetics, Humans, Kinetics, Molecular Chaperones chemistry, Oligonucleotide Array Sequence Analysis, Oncogene Protein pp60(v-src) metabolism, Phenotype, Recombinant Proteins metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae physiology, Saccharomyces cerevisiae Proteins chemistry, Adenosine Triphosphatases metabolism, HSP90 Heat-Shock Proteins metabolism, Molecular Chaperones genetics, Molecular Chaperones metabolism, Saccharomyces cerevisiae Proteins genetics, Saccharomyces cerevisiae Proteins metabolism
Abstract

Client protein activation by Hsp90 involves a plethora of cochaperones whose roles are poorly defined. A ubiquitous family of stress-regulated proteins have been identified (Aha1, activator of Hsp90 ATPase) that bind directly to Hsp90 and are required for the in vivo Hsp90-dependent activation of clients such as v-Src, implicating them as cochaperones of the Hsp90 system. In vitro, Aha1 and its shorter homolog, Hch1, stimulate the inherent ATPase activity of yeast and human Hsp90. The identification of these Hsp90 cochaperone activators adds to the complex roles of cochaperones in regulating the ATPase-coupled conformational changes of the Hsp90 chaperone cycle.

Published
2002
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28. CABYR, a novel calcium-binding tyrosine phosphorylation-regulated fibrous sheath protein involved in capacitation.

Author

Naaby-Hansen S, Mandal A, Wolkowicz MJ, Sen B, Westbrook VA, Shetty J, Coonrod SA, Klotz KL, Kim YH, Bush LA, Flickinger CJ, and Herr JC

Subjects
Amino Acid Sequence, Animals, Base Sequence, Blotting, Western, Calcium metabolism, Calcium-Binding Proteins chemistry, Calcium-Binding Proteins genetics, Cloning, Molecular, DNA, Complementary, Electrophoresis, Gel, Two-Dimensional, Fluorescent Antibody Technique, Indirect, Humans, Immune Sera, Male, Microscopy, Immunoelectron, Molecular Sequence Data, Phosphorylation, Polymorphism, Genetic, RNA Splicing, RNA, Messenger genetics, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Spermatozoa metabolism, Spermatozoa ultrastructure, Tyrosine metabolism, Calcium-Binding Proteins physiology, Phosphoproteins, Sperm Capacitation
Abstract

To reach fertilization competence, sperm undergo an incompletely understood series of morphological and molecular maturational processes, termed capacitation, involving, among other processes, protein tyrosine phosphorylation and increased intracellular calcium. Hyperactivated motility and an ability to undergo the acrosome reaction serve as physiological end points to assess successful capacitation. We report here that acidic (pI 4.0) 86-kDa isoforms of a novel, polymorphic, testis-specific protein, designated calcium-binding tyrosine phosphorylation-regulated protein (CABYR), were tyrosine phosphorylated during in vitro capacitation and bound (45)Ca on 2D gels. Acidic 86-kDa calcium-binding forms of CABYR increased during in vitro capacitation, and calcium binding to these acidic forms was abolished by dephosphorylation with alkaline phosphatase. Six variants of CABYR containing two coding regions (CR-A and CR-B) were cloned from human testis cDNA libraries, including five variants with alternative splice deletions. A motif homologous to the RII dimerization domain of PK-A was present in the N-terminus of CR-A in four CABYR variants. A single putative EF handlike motif was noted in CR-A at aas 197-209, while seven potential tyrosine phosphorylation-like sites were noted in CR-A and four in CR-B. Pro-X-X-Pro (PXXP) modules were identified in the N- and C-termini of CR-A and CR-B. CABYR localizes to the principal piece of the human sperm flagellum in association with the fibrous sheath and is the first demonstration of a sperm protein that gains calcium-binding capacity when phosphorylated during capacitation.

Published
2002
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29. Two-dimensional electrophoretic analysis of sperm antigens recognized by sperm immobilizing antibodies detected in infertile women.

Author

Shibahara H, Sato I, Shetty J, Naaby-Hansen S, Herr JC, Wakimoto E, and Koyama K

Subjects
Antigens, Surface isolation & purification, Blotting, Western, Contraception, Immunologic, Electrophoresis, Gel, Two-Dimensional, Female, Humans, Male, Membrane Proteins immunology, Membrane Proteins isolation & purification, Infertility, Female immunology, Isoantibodies blood, Isoantigens isolation & purification, Spermatozoa immunology
Abstract

In this study, high resolution two-dimensional (2-D) gel electrophoresis was used to identify human sperm antigens recognized by the sera from infertile women having sperm immobilizing (SI) antibodies. Two-D gel electrophoresis was employed to separate Percoll purified human sperm proteins using isoelectric focusing (IEF), followed by polyacrylamide gel electrophoresis (PAGE). Sperm proteins were transferred to the nitrocellulose membranes and immunoblotted with seven sera from infertile women with high titers of SI antibodies and 6 sera from those without SI antibodies. The blots were compared to the 2-D composite image of human sperm proteins [Sperm Protein Encyclopedia] and sperm surface index and the sperm surface proteins recognized by infertile sera were identified. Fifty-two human sperm surface proteins reacted with sera containing SI antibodies, while 35 of these were reactive with the SI-negative control sera. The average numbers of protein spots reacted with test and control sera were 24.6 and 15.0 respectively. A subset of sperm surface proteins which were unique to the SI antibodies were identified by the following criteria; the sperm protein spots which were highly reactive with the infertile sera containing SI antibodies but not reactive with any of the SI-negative infertile sera. The coordinates of 4 prominent immunoreactive sperm proteins were considered as possibly relevant to antibody mediated female infertility.

Published
2002
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30. Tektin B1 demonstrates flagellar localization in human sperm.

Author

Wolkowicz MJ, Naaby-Hansen S, Gamble AR, Reddi PP, Flickinger CJ, and Herr JC

Subjects
Amino Acid Sequence, Animals, Blotting, Northern, Blotting, Western, Cloning, Molecular, DNA, Complementary biosynthesis, DNA, Complementary genetics, Electrophoresis, Gel, Two-Dimensional, Escherichia coli metabolism, Female, Humans, Male, Microscopy, Fluorescence, Microtubule Proteins genetics, Microtubule Proteins immunology, Molecular Sequence Data, Oligonucleotide Probes chemical synthesis, Organ Specificity, Proteome metabolism, Rats, Rats, Inbred Lew immunology, Recombinant Proteins immunology, Recombinant Proteins metabolism, Reverse Transcriptase Polymerase Chain Reaction, Testis metabolism, Microtubule Proteins metabolism, Sperm Tail metabolism
Abstract

The human flagellar protein tektin B1 (h-tekB1) in human sperm was cloned, and its sequence and subcellular location were determined. Human sperm proteins were separated by 2-dimensional electrophoresis, and a resolved protein spot of 54 kDa with an isoelectric point (pI) of 5.3 was removed from the gel, trypsinized, and microsequenced by tandem mass spectrometry. The resulting peptides did not match any protein in the (then current) protein databases. Degenerate oligonucleotides based on the microsequences were used with a polymerase chain reaction to amplify a partial cDNA clone from human testis poly(A)(+) mRNA, and subsequently a full-length 1.5-kilobase (kb) clone (GenBank AF054910) was obtained from a testis cDNA library. The open reading frame encoded a 430-amino acid protein with 47% homology to the sea urchin tektin B1. Hybridization of labeled h-tekB1 cDNA to a multiple-tissue Northern blot demonstrated a transcript of 1.7 kb in human testis, and a multiple tissue dot-blot demonstrated high levels of expression in testis, trachea, and lung, intermediate levels in fetal brain and appendix, and low levels in ovary, pituitary, and fetal kidney. Rat polyclonal serum generated against a recombinant h-tekB1 demonstrated 3 h-tekB1 isoforms of pI 5.25, 5.5, and 5.35 at 53.5 kDa on a 2-dimensional Western blot of human sperm proteins. Immunofluorescent studies localized h-tekB1 to the principal piece of human sperm, but the endpiece was unstained.

Published
2002
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31. Co-localization of the inositol 1,4,5-trisphosphate receptor and calreticulin in the equatorial segment and in membrane bounded vesicles in the cytoplasmic droplet of human spermatozoa.

Author

Naaby-Hansen S, Wolkowicz MJ, Klotz K, Bush LA, Westbrook VA, Shibahara H, Shetty J, Coonrod SA, Reddi PP, Shannon J, Kinter M, Sherman NE, Fox J, Flickinger CJ, and Herr JC

Subjects
Acrosome metabolism, Blotting, Northern, Calcium metabolism, Calcium Channels immunology, Calcium-Binding Proteins genetics, Calcium-Binding Proteins immunology, Calreticulin, Cell Membrane metabolism, Humans, Inositol 1,4,5-Trisphosphate Receptors, Male, Microscopy, Immunoelectron, Organ Specificity, Receptors, Cytoplasmic and Nuclear immunology, Ribonucleoproteins genetics, Ribonucleoproteins immunology, Calcium Channels metabolism, Calcium-Binding Proteins metabolism, Cytoplasmic Vesicles metabolism, Receptors, Cytoplasmic and Nuclear metabolism, Ribonucleoproteins metabolism
Abstract

Modulation of the intracellular calcium concentration within mammalian spermatozoa is important in several pre-fertilization events including hyperactivated motility and the acrosome reaction. To identify calcium binding proteins (CBP) potentially regulating these processes, a (45)Ca overlay technique was employed on 2-D blots of human sperm extracts. Microsequencing by Edman degradation and CAD mass spectrometry identified a relatively abundant 60.5 kDa CBP with a pI of 4.2 as calreticulin (CRT). Immunofluorescent labelling with anti-CRT antibodies localized CRT to the acrosome, with highest fluorescence in the equatorial segment, and in the cytoplasmic droplets of 94 and 48% of human spermatozoa respectively. Double immunolabelling experiments demonstrated co-localization of CRT and the inositol 1,4,5-trisphosphate receptor (IP(3)R) in the acrosome, in the equatorial segment, and vesicular structures in the cytoplasmic droplets of the neck region. Electron microscopic immunogold labelling localized CRT to the equatorial segment of acrosome-reacted spermatozoa and to membrane-enclosed vesicles within the cytoplasmic droplet of both acrosome-intact and acrosome-reacted spermatozoa. Localization of the IP(3) receptor to the CRT-containing vesicles, in the sperm neck and to the acrosome, suggests that capacitative calcium entry in human spermatozoa may be regulated from these putative calcium storage sites.

Published
2001
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32. Differential extraction and enrichment of human sperm surface proteins in a proteome: identification of immunocontraceptive candidates.

Author

Shetty J, Diekman AB, Jayes FC, Sherman NE, Naaby-Hansen S, Flickinger CJ, and Herr JC

Subjects
Acrosome chemistry, Adult, Amino Acid Sequence, Autoantibodies blood, Autoantibodies immunology, Autoantigens analysis, Autoantigens isolation & purification, Biotinylation, Blotting, Western, Buffers, Cytoskeletal Proteins analysis, Cytoskeletal Proteins isolation & purification, Detergents, Humans, Infertility, Male blood, Infertility, Male immunology, Isoelectric Focusing, Male, Membrane Proteins analysis, Membrane Proteins isolation & purification, Molecular Sequence Data, Octoxynol, Polyethylene Glycols, Proteins analysis, Saline Solution, Hypertonic, Sequence Analysis, Protein, Solubility, Solvents, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Subtraction Technique, Succinimides, Urea, Biotin analogs & derivatives, Chemical Fractionation methods, Contraception, Immunologic, Electrophoresis, Gel, Two-Dimensional, Proteins isolation & purification, Proteome, Spermatozoa chemistry
Abstract

The objective of this study was to discover previously unknown human sperm surface proteins that may be candidate contraceptive vaccinogens. To this end, methods of concentrating human sperm proteins for microsequencing by mass spectrometry were used, which increased the likelihood of identifying surface proteins. Vectorial labeling, differential extraction and two-dimensional (2-D) gel electrophoresis were employed to identify and isolate proteins accessible at the cell surface. Percoll harvested or swim-up sperm were either solubilized directly or solubilized after surface labeling with sulfo-succinimidyl-6-(biotinamido)hexanoate (sulfo-NHS-LC-biotin). Comparisons were made of proteins extracted with four lysis buffers: (i) Celis buffer containing 9.8 M urea and 2% Igepal CA-630; (ii) 1% Triton X (TX)-100; (iii) 1.7% TX-114 followed by phase partitioning; or (iv) 1 M NaCl. Blots of proteins separated by high-resolution 2-D electrophoresis were probed with avidin and antibodies to known proteins specific for three domains: the sperm surface (SAGA-1), the acrosome (SP-10), and the cytoskeleton (alpha-tubulin). Celis buffer (45 min) extracted proteins from all three major compartments. However, a 20-s extraction in Celis buffer enriched for several proteins and enabled the identification of several novel peptides by mass spectrometry. Mild extraction with TX-100 or 1 M NaCl solubilized mainly membrane and acrosomal proteins, but not cytoskeletal proteins. Comparison of biotinylated proteins extracted by each method showed that the major vectorially labeled proteins solubilized by Celis buffer were also solubilized by TX-100, TX-114, and 1 M NaCl. Extraction with TX-114 followed by phase-partitioning significantly enriched hydrophobic surface proteins and aided resolution and isolation. Eight protein spots microsequenced following all these extraction methods proved to be novel sperm molecules.

Published
2001
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33. Proteomics--post-genomic cartography to understand gene function.

Author

Naaby-Hansen S, Waterfield MD, and Cramer R

Subjects
Animals, Electrophoresis, Gel, Two-Dimensional methods, Electrophoresis, Gel, Two-Dimensional trends, Humans, Mass Spectrometry methods, Mass Spectrometry trends, Peptide Mapping trends, Sequence Tagged Sites, Signal Transduction physiology, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization trends, Peptide Mapping methods, Proteome analysis, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods
Abstract

The completion of the genomic sequences of numerous organisms from human and mouse to Caenorhabditis elegans and many microorganisms, and the definition of their genes provides a database to interpret cellular protein-expression patterns and relate them to protein function. Proteomics technologies that are dependent on mass spectrometry and involve two-dimensional gel electrophoresis are providing the main window into the world of differential protein-expression analysis. In this article, the limitations and expectations of this research field are examined and the future of the analytical needs of proteomics is explored.

Published
2001
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34. Analysis of ribonucleases following gel electrophoresis.

Author

Scadden AD and Naaby-Hansen S

Subjects
Electrophoresis, Gel, Two-Dimensional methods, Electrophoresis, Polyacrylamide Gel methods, Indicators and Reagents, RNA chemistry, RNA metabolism, Ribonucleases isolation & purification, Substrate Specificity, Ribonucleases analysis
Published
2001
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35. Differential nuclear localization of the cancer/testis-associated protein, SPAN-X/CTp11, in transfected cells and in 50% of human spermatozoa.

Author

Westbrook VA, Diekman AB, Naaby-Hansen S, Coonrod SA, Klotz KL, Thomas TS, Norton EJ, Flickinger CJ, and Herr JC

Subjects
Amino Acid Sequence, Animals, Blotting, Western, Cell Line, Cytoplasm chemistry, Fluorescent Antibody Technique, Indirect, Humans, Isoelectric Point, Male, Molecular Sequence Data, Molecular Weight, Nuclear Envelope chemistry, Nuclear Proteins chemistry, Solubility, Spermatozoa ultrastructure, Vacuoles chemistry, X Chromosome, Y Chromosome, Cell Nucleus chemistry, Nuclear Proteins analysis, Spermatozoa chemistry, Transfection
Abstract

Cancer-testis antigens (CTAs) represent potential targets for cancer immunotherapy because these proteins are widely distributed in tumors but not in normal tissues, except testes. In this paper, we identify homology of the CTA CTp11 with SPAN-X (sperm protein associated with the nucleus mapped to the X chromosome). On two-dimensional Western blots of human sperm extracts, SPAN-X antibodies recognized 19 spots ranging from 20 to 23 kDa with isoelectric points from 5.0 to 5.5. Differential extraction of spermatozoa demonstrated that the SPAN-X protein is highly insoluble. Only 50% of ejaculated spermatozoa exhibited SPAN-X immunofluorescent staining. Dual localization of the sex chromosomes and the SPAN-X protein demonstrated that an equal number of X- and Y-bearing spermatozoa exhibited SPAN-X staining. In transfected mammalian CV1 cells, the SPAN-Xa and SPAN-Xb proteins were localized to the nucleus and cytoplasm, respectively, by indirect immunofluorescence. On immunoblots of CV1 cells, the SPAN-Xa protein migrated at 15-20 kDa, whereas the SPAN-Xb protein migrated at a higher molecular weight of 21-22 kDa. The SPAN-X protein was ultrastructurally associated with nuclear vacuoles and the redundant nuclear envelope. SPAN-X is the first protein specifically localized to these poorly characterized structures of the mammalian sperm nucleus and provides a unique biochemical marker for investigation of their function in spermatozoa as well as the role of SPAN-X/CTp11 in human tumors.

Published
2001
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36. Anti-sperm antibodies from infertile patients and their cognate sperm antigens: a review. Identity between SAGA-1, the H6-3C4 antigen, and CD52.

Author

Diekman AB, Norton EJ, Westbrook VA, Klotz KL, Naaby-Hansen S, and Herr JC

Subjects
Animals, CD52 Antigen, Female, Humans, Male, Antigens, CD immunology, Antigens, Neoplasm, Antigens, Surface immunology, Autoantibodies analysis, Glycoproteins immunology, Infertility, Female immunology, Infertility, Male immunology, Isoantibodies analysis, Spermatozoa immunology
Abstract

Problem: The correlation of anti-sperm antibodies (ASA) with some instances of unexplained infertility implicates a role for these antibodies in blocking fertilization. Improved diagnosis and treatment of immunologic infertility, as well as a more complete understanding of the mechanism behind this phenomenon, are dependent on the identification and characterization of relevant sperm antigens., Method of Study: In this article, we review literature on methods employed to identify sperm antigens using anti-sperm polyclonal and monoclonal antibodies from infertile patients and vasectomized men. Particular focus is given to approaches using human and mouse monoclonal antibodies to define the SAGA-1 human sperm antigen., Results: ASA present in sera and genital tract secretions from infertile patients and vasectomized men have been employed in a variety of methods to identify sperm antigens. In an alternate approach, a monoclonal antibody (mAb), H6-3C4, was immortalized from the lymphocytes of an infertile woman who exhibited sperm-immobilizing titers. Subsequently, the sperm-agglutinating, murine S19 mAb was shown to react with the H6-3C4 cognate antigen. The H6-3C4 S19 cognate antigen, designated Sperm Agglutination Antigen-1 (SAGA-1), was characterized as a polymorphic, highly acidic, GPI-anchored glycoprotein on the surface of human spermatozoa. Purification with the S19 mAb followed by microsequencing demonstrated that the SAGA-1 core peptide is identical to CD52, a glycoprotein on the surface of human lymphocytes. Immunoblot analysis demonstrated that these two glycoproteins differed in carbohydrate composition. Thus, sperm SAGA-1 and lymphocyte CD52 represent glycoforms, glycoproteins with the same core peptide but with different carbohydrate structures., Conclusions: Autoimmunity to the SAGA-1 and/or CD52 glycoforms may lead to infertility. Structural and immunologic differences between these glycoproteins may be important factors in the etiology of immunologic infertility and other autoimmune disorders.

Published
2000
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37. PI-PLC releases a 25-40 kDa protein cluster from the hamster oolemma and affects the sperm penetration assay.

Author

Coonrod S, Naaby-Hansen S, Shetty J, and Herr J

Subjects
Animals, Biotinylation, Cricetinae, Egg Proteins metabolism, Electrophoresis, Gel, Two-Dimensional, Female, Humans, Male, Molecular Weight, Oocytes metabolism, Ovum drug effects, Phosphatidylinositol Diacylglycerol-Lyase, Phosphoinositide Phospholipase C, Sequence Analysis, Spermatozoa physiology, Oocytes drug effects, Sperm-Ovum Interactions drug effects, Spermatozoa drug effects, Type C Phospholipases pharmacology
Abstract

The effects of phosphatidylinositol-specific phospholipase C (PI-PLC) on human sperm-hamster oocyte interaction were investigated to determine whether PI-PLC cleavable glycosylphosphatidyinositol (GPI)-anchored proteins are involved in sperm-egg binding and fusion. Two-dimensional electrophoresis was then utilized to visualize proteins released from hamster oocytes following PI-PLC treatment. For the binding and fusion assay, either spermatozoa or eggs were treated with 1 IU/ml PI-PLC for 30 min and washed prior to gamete co-incubation. Treatment of human spermatozoa with PI-PLC significantly (P

Published
1999
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38. FSP95, a testis-specific 95-kilodalton fibrous sheath antigen that undergoes tyrosine phosphorylation in capacitated human spermatozoa.

Author

Mandal A, Naaby-Hansen S, Wolkowicz MJ, Klotz K, Shetty J, Retief JD, Coonrod SA, Kinter M, Sherman N, Cesar F, Flickinger CJ, and Herr JC

Subjects
Amino Acid Sequence, Blotting, Northern, Blotting, Southern, Cloning, Molecular, DNA, Complementary analysis, Escherichia coli metabolism, Humans, In Vitro Techniques, Infertility immunology, Male, Molecular Sequence Data, Molecular Weight, Phosphorylation, Proteins isolation & purification, Recombinant Proteins biosynthesis, Recombinant Proteins isolation & purification, Spermatozoa immunology, Testis immunology, Tyrosine immunology, Proteins metabolism, Sperm Capacitation physiology, Spermatozoa metabolism, Testis metabolism, Tyrosine metabolism
Abstract

Protein tyrosine phosphorylation has been associated with both capacitation and motility of mammalian sperm. During capacitation, human spermatozoa undergo tyrosine phosphorylation of a characteristic set of proteins, only one of which has thus far been cloned and localized. We report here the sequence of a fibrous sheath protein of 95 kDa (FSP95) that undergoes tyrosine phosphorylation during capacitation of human spermatozoa and has similarity to sperm A-kinase anchor proteins (AKAPs). FSP95 is both auto- and iso-antigenic in humans as it is recognized by sera containing antisperm antibodies from infertile men and women. The 853-residue protein has a calculated molecular weight of 94.6 kDa and an isoelectric point (pI) of 6.0, and it contains multiple potential phosphorylation sites for protein kinase C and casein kinase II as well as one potential tyrosine kinase phosphorylation site at amino acid 435. The sequence has amino acid homology to mouse sperm fibrous sheath AKAP82 (pro-mAKAP82, 34% identity) and to human sperm fibrous sheath AKAP82 (pro-hAKAP82, 32% identity). The gene encoding FSP95 has 5 exons separated by 4 introns and is located on chromosome 12 at locus p13.3. Northern analysis detected a single transcript of approximately 3.0 kilobases, and Northern dot blot analysis of 50 human tissues revealed FSP95 mRNA expression only in testis. By employing sperm immobilization, indirect immunofluorescence, and immunoelectron microscopy with antisera to purified recombinant FSP95, the protein was localized to the ribs of the fibrous sheath in the principal piece of the sperm tail. FSP95 is the second fibrous sheath protein to be cloned, sequenced and localized in human spermatozoa.

Published
1999
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39. N-linked glycan of a sperm CD52 glycoform associated with human infertility.

Author

Diekman AB, Norton EJ, Klotz KL, Westbrook VA, Shibahara H, Naaby-Hansen S, Flickinger CJ, and Herr JC

Subjects
Antibodies, Monoclonal immunology, Antibody Specificity, Autoantibodies immunology, CD52 Antigen, Female, Humans, Male, Antigens, CD immunology, Antigens, Neoplasm, Antigens, Surface immunology, Glycoproteins immunology, Infertility, Female immunology, Spermatozoa immunology
Abstract

In a benchmark study, Isojima and colleagues established H6-3C4, the first successful heterohybridoma immortalized from the peripheral blood lymphocytes of an infertile woman who exhibited high sperm-immobilizing antibody titers. The present report demonstrates the identity between the glycoprotein antigens recognized by the human H6-3C4 monoclonal antibody (mAb) and the murine S19 mAb, generated in our laboratory to sperm agglutination antigen-1 (SAGA-1). Both mAb's recognize N-linked carbohydrate epitopes on the 15-25 kDa, polymorphic SAGA-1 glycoprotein that is localized to all domains of the human sperm surface. Treatment with phosphatidylinositol-specific phospholipase C demonstrated that SAGA-1 is anchored in the sperm plasmalemma via a GPI-lipid linkage. Immunoaffinity purification and microsequencing indicated that the core peptide of the SAGA-1 glycoprotein is identical to the sequence of CD52, a GPI-anchored lymphocyte differentiation marker implicated in signal transduction. Comparison of anti-SAGA-1 and anti-CD52 immunoreactivities revealed that the sperm form of CD52 exhibits N-linked glycan epitopes, including the epitope recognized by the infertility-associated H6-3C4 mAb, which are not detected on lymphocyte CD52. Thus, the two populations of the CD52 glycoprotein on lymphocytes and spermatozoa represent glycoforms, glycoprotein isoforms with the same core amino acid sequence but different carbohydrate structures. Furthermore, mAb's to the unique carbohydrate epitopes on sperm CD52 have multiple inhibitory effects on sperm function, including a cytotoxic effect on spermatozoa in the presence of complement. These results are the first to implicate unique carbohydrate moieties of a sperm CD52 glycoform as target epitopes in the anti-sperm immune response of an infertile woman. Furthermore, localization of CD52 on all domains of the sperm surface coupled with the multiple sperm-inhibitory effects of antibodies to its unique carbohydrate moieties suggest opportunities for immunocontraceptive development.

Published
1999
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40. Human sperm proteome: immunodominant sperm surface antigens identified with sera from infertile men and women.

Author

Shetty J, Naaby-Hansen S, Shibahara H, Bronson R, Flickinger CJ, and Herr JC

Subjects
Blotting, Western, Electrophoresis, Polyacrylamide Gel, Female, Humans, Hydrogen-Ion Concentration, Immunoglobulin G blood, Immunoglobulin M blood, Isoelectric Focusing, Luminescent Measurements, Male, Proteins analysis, Proteins immunology, Sex Characteristics, Antigens, Surface analysis, Immune Sera immunology, Infertility, Female immunology, Infertility, Male immunology, Spermatozoa immunology
Abstract

The objective of this study was to identify those immunodominant sperm antigens recognized by antisperm antibodies (ASA) in the serum samples of infertile men and women. High-resolution two-dimensional gel electrophoresis was employed to separate human sperm proteins using isoelectric focusing or nonequilibrium pH gradient electrophoresis, followed by PAGE. Serum samples from 15 infertile male subjects and 6 infertile female subjects that contained ASA as assayed by the immunobead binding test (IBT) were analyzed by Western blotting followed by enhanced chemiluminescence (ECL). Serum samples from 10 fertile subjects (5 males and 5 females) that were ASA negative by IBT were used as controls. The ECL blots were analyzed by computer scanning to compare the immunoreactivity between serum samples from fertile and infertile subjects and to identify the antigens unique to the sera of the infertile subjects; 98 sperm auto- and iso-antigenic protein spots were recognized by sera from infertile males and females but not from fertile subjects. Based on vectorial labeling with 125I at the sperm surface, a subset of 6 auto- and iso-antigens was identified as possibly relevant to antibody-mediated infertility.

Published
1999
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41. Post-obstruction rat sperm autoantigens identified by two-dimensional gel electrophoresis and western blotting.

Author

Flickinger CJ, Bush LA, Williams MV, Naaby-Hansen S, Howards SS, and Herr JC

Subjects
Animals, Female, Male, Rats, Rats, Inbred Lew, Vasectomy, Autoantigens analysis, Blotting, Western methods, Electrophoresis, Gel, Two-Dimensional methods, Spermatozoa immunology
Abstract

Although antisperm autoantibody responses to obstruction of the male reproductive system have been documented, information on the nature of the cognate sperm autoantigens has been limited. In the present study, the patterns of sperm autoantigens recognized by sera from rats after obstruction of the vas deferens or epididymis were studied by high resolution two-dimensional (2-D) gel electrophoresis and western blotting. Comparisons of patterns of autoantigens stained on 2-D western blots of sera from prepubertal vasectomy, prepubertal epididymal ligation and adult vasectomy groups revealed both similarities and differences. Sera from sham-operated animals showed no detectable reaction or much lighter staining of a small number of spots. Visualization of sperm autoantigens on 2-D western blots supported the hypothesis that there is a relatively small set of sperm proteins that can be regarded as dominant post-obstruction sperm autoantigens because they are recognized by multiple post-obstruction sera. The 2-D analysis revealed previously undetected distinctions in the autoantigens recognized after adult and prepubertal vasectomy, as well as variations with the site of obstruction. These differences in the response may be due in part to changes in antigens of spermatozoa in different parts of the tract and at different ages, as well as variations in exposure of sperm cell proteins to the immune system resulting from the sites of spermatic granulomas. Preparative 2-D gels and western blotting with post-obstruction sera are now being used to identify specific sperm autoantigens by microsequencing of selected proteins.

Published
1999
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42. Treatment of mouse oocytes with PI-PLC releases 70-kDa (pI 5) and 35- to 45-kDa (pI 5.5) protein clusters from the egg surface and inhibits sperm-oolemma binding and fusion.

Author

Coonrod SA, Naaby-Hansen S, Shetty J, Shibahara H, Chen M, White JM, and Herr JC

Subjects
Animals, Biotinylation, Calcimycin pharmacology, Calcium pharmacology, Cell Adhesion physiology, Female, Fertilization physiology, Glycosylphosphatidylinositols metabolism, In Vitro Techniques, Integrin alpha6beta1, Integrins immunology, Male, Meiosis drug effects, Mice, Oocytes drug effects, Phosphatidylinositol Diacylglycerol-Lyase, Phosphoinositide Phospholipase C, Zona Pellucida metabolism, Membrane Fusion physiology, Membrane Glycoproteins metabolism, Oocytes metabolism, Spermatozoa metabolism, Type C Phospholipases pharmacology
Abstract

The effect of phosphatidyinositol-specific phospholipase C (PI-PLC) on mouse sperm-egg interaction was investigated in this study to determine if glycosyl-phosphatidylinositol (GPI)-anchored proteins are involved in mammalian fertilization. When both sperm and zona-intact oocytes were pretreated with a highly purified preparation of PI-PLC and coincubated, there was no significant effect on sperm-zona pellucida binding; however, fertilization was reduced from 59.6% (control group) to 2.8% (treatment group). A similar reduction in fertilization rates was found when zona-intact oocytes were treated with PI-PLC and washed prior to incubation with untreated sperm. The effect of PI-PLC on sperm binding and fusion with zona-free oocytes was then investigated. Treatment of sperm with PI-PLC had no significant effect on sperm-egg binding or fusion. However, treatment of eggs with PI-PLC significantly reduced sperm-egg binding and fusion from 6.2 bound and 2.1 fused sperm per egg in the control group to 2.1 bound and 0.02 fused sperm per egg in the treatment group. This decrease in sperm-egg binding and fusion depended on the dose of PI-PLC employed, with a maximal inhibitory effect on binding and fusion at 5 and 1 U/ml, respectively. PI-PLC-treated oocytes could be artificially activated by calcium ionophore, demonstrating that the oocytes were functionally viable following treatment. Furthermore, treatment of oocytes with PI-PLC did not reduce the immunoreactivity of the non-GPI-anchored egg surface integrin, alpha6beta1. Taken together, these observations support the hypothesis that PI-PLC affects fertilization by specifically releasing GPI-anchored proteins from the oolemma. In order to identify the oolemmal GPI-anchored proteins involved in fertilization, egg surface proteins were labeled with sulfo-NHS biotin, treated with PI-PLC, and analyzed by two-dimensional gel electrophoresis followed by avidin blotting. A prominent high-molecular-weight protein cluster (approximately 70 kDa, pI 5) and a lower molecular weight (approximately 35-45 kDa, pI 5.5) protein cluster were released from the oolemmal surface as a result of PI-PLC treatment. It is likely that these GPI-anchored egg surface proteins are required for sperm-egg binding and fusion., (Copyright 1999 Academic Press.)

Published
1999
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43. Immunological response in the primate oviduct to a defined recombinant sperm immunogen.

Author

Kurth BE, Bryant D, Naaby-Hansen S, Reddi PP, Weston C, Foley P, Bhattacharya R, Flickinger CJ, and Herr JC

Subjects
Animals, Fallopian Tubes metabolism, Female, Humans, Immunization, Male, Membrane Proteins, Models, Immunological, Primates immunology, Spermatozoa, Vaccines, Acrosome, Antigens, Antigens, Surface immunology, Fallopian Tubes immunology, Gonadal Steroid Hormones, Proteins immunology
Abstract

Assessment of immune responses in the oviduct is of importance in understanding reproductive tract responses to infections, vaccination against reproductive tract pathogens, or contraceptive immunogens. This review discusses a technique that permits repeated sampling of oviductal fluid from the same monkey at intervals spanning up to several years, and the analysis of antigen-specific immunoglobulins in the fluid. This technique is important to immunocontraceptive development because previous studies in primates have lacked information on oviductal immune responses and contraceptive efficacy may not correlate well with serum antibody titers. Thus, a reliable method of sampling oviductal fluid before and after immunization with a defined antigen is required to determine the quantity and type of local immune responses necessary to achieve contraceptive effects. Implantation of access ports proved useful for repeatedly aspirating oviductal fluid in vivo from cynomolgus monkeys that was free from artifactual contaminants and with no observable changes in the behavior or health of the animals. Subsequent assays of relative and absolute concentrations of antibodies in oviductal fluid and serum demonstrated the presence of IgA and IgG specific for the recombinant sperm immunogen SP-10 in fluid collected from the periovulatory oviduct of primates after intramuscular inoculations. The antibodies evoked by the recombinant sperm vaccinogen recognized the endogenous antigen target on both human and macaque sperm, lending support for the possibility of developing a contraceptive immunogen that prevents fertilization.

Published
1997
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44. Biochemical characterization of sperm agglutination antigen-1, a human sperm surface antigen implicated in gamete interactions.

Author

Diekman AB, Westbrook-Case VA, Naaby-Hansen S, Klotz KL, Flickinger CJ, and Herr JC

Subjects
Antibodies, Monoclonal immunology, Antigens, Surface chemistry, Antigens, Surface immunology, Detergents pharmacology, Electrophoresis, Polyacrylamide Gel, Fluorescent Antibody Technique, Direct, Humans, Immunoblotting, In Vitro Techniques, Male, Membrane Glycoproteins chemistry, Membrane Glycoproteins immunology, Microscopy, Fluorescence, Periodic Acid, Semen drug effects, Semen immunology, Semen physiology, Spermatozoa drug effects, Spermatozoa physiology, Antigens, Surface metabolism, Membrane Glycoproteins metabolism, Sperm Agglutination immunology, Spermatozoa immunology
Abstract

The anti-sperm monoclonal antibody (mAb) S19 was previously demonstrated to agglutinate human spermatozoa, inhibit sperm penetration of cervical mucus, and inhibit sperm-zona pellucida binding. These results implicated the cognate S19 antigen, designated sperm agglutination antigen-1 (SAGA-1), in gamete interactions and identified SAGA-1 as an attractive candidate for immunocontraceptive development. In the present study, evaluation of sperm agglutination with video microscopy showed that the S19 mAb rapidly and completely agglutinated human spermatozoa in a "tangled" pattern of agglutination. One- and two-dimensional immunoblot analyses identified SAGA-1 as a highly acidic, polymorphic sperm protein with an apparent molecular mass of 15-25 kDa and an isoelectric point of 2.5-3.0. Periodate treatment abolished this immunoreactivity, demonstrating that the S19 mAb reacted with a carbohydrate epitope and indicating that SAGA-1 is a glycoprotein. Absence of S19 immunoreactivity in postvasectomy seminal fluid implicated the testis, epididymis, and/or proximal vas deferens in the expression of SAGA-1. In solubility and phase partitioning assays, SAGA-1 was extracted from spermatozoa in Triton X-114 and exhibited the hydrophobic characteristics of integral and glycosylphosphatidyl inositol-anchored membrane proteins. These results identify SAGA-1 as a hydrophobic, highly acidic sperm glycoprotein that is localized on the entire sperm surface and has potential significance as a target for antibodies that inhibit sperm function and gamete interactions.

Published
1997
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45. A novel negative imaging technique for accurate localization of stainable proteins on complex two-dimensional autoradiograms.

Author

Naaby-Hansen S, Roof RW, Flickinger CJ, Grafer CM, Parsons SJ, and Herr JC

Subjects
Animals, Electrophoresis, Polyacrylamide Gel, Fibroblasts chemistry, Humans, Immunoblotting, Iodine Radioisotopes, Isoelectric Focusing, Male, Mice, Phosphoproteins analysis, Phosphorus Radioisotopes, Spermatozoa chemistry, Tubulin analysis, Autoradiography methods, Electrophoresis, Gel, Two-Dimensional, Proteins analysis
Abstract

This paper describes a fast, simple, and accurate method for localization of protein antigens in complex two-dimensional (2-D) autoradiograms where the precise position and identity of the protein is required. The method involves the creation of negative images on an autoradiogram through arrangement of image-intensifying screens. By placing a chromogenically stained 2-D gel or blot between the intensifying screen and the film, photons emitted from the intensifying screen are obstructed by the stained spots, thus creating a negative image on the film. The technique can be used in autoradiograms of proteins labeled with either 32P or (125)I radioisotopes. The technique permits analysis of radiolabeled, gold-stained and immunoreacted proteins on a single film and offers versatility by combining analysis of total protein patterns with specific identification of radiolabeled and/or immunoreacted protein spots. The technique is especially useful when selecting a subset of specifically radiolabeled proteins from the total protein pattern in 2-D gels or membranes for microsequencing.

Published
1997
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46. Two-dimensional gel electrophoretic analysis of vectorially labeled surface proteins of human spermatozoa.

Author

Naaby-Hansen S, Flickinger CJ, and Herr JC

Subjects
Biotin, Blood Proteins chemistry, Electrophoresis, Polyacrylamide Gel, Humans, Image Processing, Computer-Assisted, Immunoblotting, Iodine Radioisotopes, Isoelectric Focusing, Male, Semen chemistry, Silver Staining, Solubility, Membrane Proteins chemistry, Spermatozoa chemistry
Abstract

The objective of this study was to identify the repertoire of proteins exposed on the surface of ejaculated human spermatozoa. High-resolution two-dimensional gel systems for separation of human sperm and seminal plasma proteins were developed using both isoelectric focusing (IEF) and nonequilibrium pH gradient electrophoresis (NEPHGE) followed by polyacrylamide gel electrophoresis (IEF/PAGE, NEPHGE/PAGE). Proteins were visualized by silver staining of gels and by electroblotting followed by gold staining. The protein patterns were analyzed by computer after laser or camera scanning. One thousand three hundred ninety-seven sperm proteins with a molecular mass between 5 and 160 kDa and isoelectric points (pI) from 4 to 11 were catalogued from silver-stained gels loaded with approximately 0.25 mg of NP-40/urea extracts of sperm harvested by Percoll density gradient centrifugation, and 1191 proteins were resolved following extraction with SDS/3-[3-cholamidopropyl) dimethylammonio]-1-propane-sulfonate/urea. Analysis of seminal plasma proteins obtained from vasectomized patients revealed over 300 silver-stained proteins, which aided the identification of sperm-coating proteins acquired from secretions of the accessory sex organs. Sperm surface proteins accessible to vectorial labeling with 125I or N-hydroxysuccinimide biotin were identified; 181 protein spots were radiolabeled with 125I, while 228 protein spots were biotinylated, including several groups of protein isoforms. Cytoskeletal and intra-acrosomal control proteins were not iodinated or biotinylated, thus verifying the surface specificity of both labeling methods. Ninety-eight sperm surface proteins were labeled by both iodine and biotin, and 22 sperm surface proteins, representing five groups of protein isoforms, were shown to contain phosphotyrosine. A composite computer image showing the position of the dually vectorially labeled sperm surface proteins was constructed, together with a table of the proteins' molecular weight, pI, and relative concentration. In addition, novel isoforms of actin, beta-tubulin, PH-20, and several phosphotyrosine-containing proteins were identified in human sperm.

Published
1997
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47. Complementary deoxyribonucleic acid cloning and characterization of mSP-10: the mouse homologue of human acrosomal protein SP-10.

Author

Reddi PP, Naaby-Hansen S, Aguolnik I, Tsai JY, Silver LM, Flickinger CJ, and Herr JC

Subjects
Amino Acid Sequence, Animals, Antigens chemistry, Base Sequence, Chromosome Mapping, Electrophoresis, Gel, Two-Dimensional, Escherichia coli genetics, Gonadal Steroid Hormones chemistry, Humans, Immunoblotting, Membrane Proteins, Mice, Molecular Sequence Data, Polymorphism, Restriction Fragment Length, Recombinant Proteins immunology, Recombinant Proteins isolation & purification, Sequence Analysis, Sequence Homology, Acrosome, Antigens genetics, Cloning, Molecular, DNA, Complementary chemistry, Gonadal Steroid Hormones genetics
Abstract

Complementary DNA encoding the putative mouse homologue for human acrosomal protein SP-10, a candidate contraceptive vaccinogen, was cloned and sequenced. The entire open reading frame (amino acids 18 to 261) of the mouse SP-10 (mSP-10), with the exception of the signal peptide (amino acids 1 to 17), was placed under the influence of inducible T7 RNA polymerase/promoter system to overproduce recombinant protein (re-mSP-10) in Escherichia coli. A six-histidine tag, which was coexpressed at the carboxyl terminus of re-mSP-10, provided the means for purification of re-mSP-10 by immobilized metal chelation affinity chromatography technique. The level of purity of re-mSP-10 thus obtained was determined by 2-dimensional gel electrophoresis to be 98%. Immunoblotting with monoclonal and polyclonal antibodies previously generated against human or baboon SP-10 showed that mSP-10 shared significant antigenic similarity with its primate counterparts. The position of mSP-10 in the mouse genome was next mapped through segregation analysis of an interspecific backcross panel of 96 animals. Acrv1 (assigned gene symbol for mSP-10) was localized in the proximal portion of mouse chromosome 9 in a region that exhibits synteny with human 11q23, the region to which ACRV1 (gene symbol for human SP-10) was previously mapped. These characterizations by combined immunological and gene mapping techniques established the cloned mSP-10 to be the mouse homologue of SP-10.

Published
1995
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48. The humoral autoimmune response to vasectomy described by immunoblotting from two-dimensional gels and demonstration of a human spermatozoal antigen immunochemically crossreactive with the D2 adhesion molecule.

Author

Naaby-Hansen S

Subjects
Adolescent, Adult, Antigens analysis, Cell Adhesion Molecules, Neuronal immunology, Cross Reactions, Electrophoresis, Gel, Two-Dimensional, Female, Humans, Immunoblotting, Male, Autoantibodies analysis, Spermatozoa immunology, Vasectomy adverse effects
Abstract

The specificity of human serum antispermatozoal antibodies was analysed by immunoblotting after two-dimensional electrophoretic separation (IEF/PAGE) of human spermatozoal proteins. Spermatozoal proteins with Mr 20-200 kDa and pI between 4.5 and 7.8 were analysed for antigenicity. Fifteen sera (four female and 11 male) were analysed for antisperm IgG antibodies. Individual IgG binding patterns were observed. The antisperm antibody response to ligation of the vas deferens was described by immunoblotting analysis of sera taken pre- and post-operatively at regular intervals from three men undergoing vasectomy. The high resolution of spermatozoal antigens allowed a specific description of the humoral response to vasectomy. Both appearance and disappearance of spots were observed in the postoperative period, indicating induction of new antibody producing clones and binding of former free antibodies in circulating immunocomplexes. In one patient five glycosylated proteins induced an IgM response 2 weeks after vasectomy. Four of these autoantigens with Mr of 122 kDa, 119 kDa, 104 kDa and 77 kDa and pI of 5.9, 6.1, 7.7 and 6.0, respectively, have previously been shown to be intrinsic membrane proteins (Naaby-Hansen, (1990) J., Reprod. Immunol. 17). An observed immunochemical crossreactivity between the interneuronal adhesion molecule, D2-protein and an antigen extracted from human sperm and teratomas is discussed.

Published
1990
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49. Electrophoretic map of acidic and neutral human spermatozoal proteins.

Author

Naaby-Hansen S

Subjects
Affinity Labels, Azirines, Borohydrides, Electrophoresis, Gel, Two-Dimensional, Electrophoresis, Polyacrylamide Gel, Humans, Iodine Radioisotopes, Isoelectric Focusing, Lectins metabolism, Male, Membrane Glycoproteins analysis, Solubility, Tritium, Membrane Proteins analysis, Spermatozoa chemistry
Abstract

A high resolution two dimensional electrophoretic technique (2-D), isoelectric focusing followed by polyacrylamide gel electrophoresis, for separation of neutral and acidic human spermatozoal proteins was established. Silver stained 2-D gels revealed over 260 proteins with Mr 20-200 kDa and pI between 4.5 and 7.8. Membrane proteins were radio-iodinated in their hydrophobic cores with the hydrophobic photoactivatable reagent 3 (trifluoromethyl)-3-(m-[125I]iodophenyl) diazirine (TID). Externally exposed carbohydrate side chains were radiolabelled by NaB(3H)4 reduction. 2-D lectin blotting was performed with horseradish peroxidase conjugated Concanavalin A (Con A), biotinylated Vicia faba agglutinin (VFA) and Solanum tuberosum agglutinin (STA). A map of 258 human spermatozoal proteins is presented and 48 TID-labelled proteins have been biochemically characterized.

Published
1990
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50. Autoantibodies against spermatozoal antigens detected by immunoblotting and agglutination. A longitudinal study of vasectomized males.

Author

Hald J, Naaby-Hansen S, Egense J, Hjort T, and Bjerrum OJ

Subjects
Adult, Agglutination Tests, Autoantibodies immunology, Binding Sites, Antibody, Collodion, Electrophoresis, Polyacrylamide Gel, Epitopes analysis, Humans, Longitudinal Studies, Male, Middle Aged, Autoantibodies analysis, Sperm Agglutination, Spermatozoa immunology, Vasectomy
Abstract

Sera taken pre- and post-operatively at regular intervals within a year from 16 men undergoing vasectomy were analysed for autoantibodies against spermatozoal proteins by immunoblotting. The reaction patterns were compared with the results of sperm agglutination tests. Immunoblotting revealed the presence of autoantibodies against various spermatozoal polypeptides in all sera taken pre-operatively and post-operatively. On average, seven polypeptides showed reaction. During the post-operative period two patients developed spermatozoal agglutinins in moderate titers (greater than 16) but in immunoblotting no change in band reactivity was observed for these two patients. However, scanning of the immunoblotting results revealed that one of the patients, although without sperm agglutinins, during the post-operative period showed an increasing band colouring of a polypeptide of Mr 31,500, reflecting an increased level of the corresponding antibodies.

Published
1987
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