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2. Stage-specific apoptosis of male germ cells in the rat: mechanisms of cell death studied by supravital squash preparations

Author

M. Parvinen and K. Henriksén

Subjects
Male, Programmed cell death, Somatic cell, Apoptosis, Biology, Specimen Handling, Rats, Sprague-Dawley, chemistry.chemical_compound, Spermatocytes, Annexin, medicine, Animals, Microscopy, Phase-Contrast, Testosterone, Propidium iodide, Annexin A5, Cells, Cultured, Fluorescent Dyes, Mesylates, Staining and Labeling, Leydig Cells, Cell Biology, General Medicine, Spermatids, Spermatozoa, Spermatogonia, Rats, Cell biology, Chromatin, Meiosis, medicine.anatomical_structure, chemistry, Transillumination, Spermatogenesis, Fluorescein-5-isothiocyanate, Germ cell, Propidium, Developmental Biology
Abstract

Apoptosis has been proposed as a mechanism by which testis germ cells are removed during normal and various pathological conditions. To establish a new rapid way to detect stage-specific apoptosis in male rat germ cells, their supravital morphology was examined from carefully squashed monolayers of living cells, after several established toxic treatments, using a phase contrast microscope. The results were compared with early detection of apoptosis using annexin V and propidium iodide (PI) stainings. The apoptosis of type-A spermatogonia and round spermatids proceeded in a similar way to somatic cells, while intermediate and type-B spermatogonia, and particularly the dividing spermatocytes, possessed characteristics not entirely typical for apoptosis. Death of elongated spermatids was difficult to assess owing to their compacted chromatin. As the first phases of degeneration seemed different in various germ cell classes, the final stage (karyopycnosis) was similar for most cells. Degenerating cells also showed positive reactions for annexin V and PI. The ‘living cell method’ provides rapid and accurate possibilities for analysis of stage-specific apoptosis during spermatogenesis. This method is not influenced by artefacts induced by fixation, embedding and sectioning. It may be developed further for routine analyses of the accurate stage-specific effects of various physical and chemical effects on mammalian and human spermatogenesis.

Published
1998
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3. Histochemical tracing of zinc ions in the rat testis

Author

Gorm Danscher, M Parvinen, Meredin Stoltenberg, Erik Ernst, Michael Busk Sørensen, and K Henriksén

Subjects
Male, Silver Staining, Embryology, medicine.medical_specialty, chemistry.chemical_element, Zinc, Sulfides, Biology, Testicle, Rats, Sprague-Dawley, Internal medicine, Testis, Genetics, medicine, Animals, Rats, Wistar, Spermatogenesis, Acrosome, Molecular Biology, Chelating Agents, Endoplasmic reticulum, Leydig Cells, Obstetrics and Gynecology, Cell Biology, Seminiferous Tubules, Spermatozoa, Molecular biology, Rats, Meiosis, Endocrinology, Seminiferous tubule, medicine.anatomical_structure, Reproductive Medicine, chemistry, Cytoplasm, Sperm Tail, Ultrastructure, Ditiocarb, Developmental Biology
Abstract

To detect free zinc ions in the rat testes four rats were transcardially perfused with Na2S, and the seminiferous tubules from two other rats were incubated in Na2S. Sections from the two sources were autometallographically (AMG) developed, whereby zinc sulphide crystal lattices created in the tissue by the sulphide treatment were silver enhanced. Light microscopical analysis showed zinc ions in primary spermatogonia until the zygotene primary spermatocytes (stage I), in late pachytene spermatocytes (stages XII and XIII), and in late spermatids from step 15 to step 19 (stages I-VIII). The highest intensity of AMG grains was detected in the residual bodies and tails of step 19 spermatids. Grains were occasionally found in the cytoplasm of Leydig cells. Sections from animals treated with the chelator diethyldithiocarbamate prior to sulphide treatment showed a complete lack of AMG staining. At ultrastructural levels the AMG grains were found in smooth-surfaced endoplasmic reticulum of all spermatogonial stages, and in the acrosome, midpiece, and tail of late spermatids. The presence of zinc ions in preleptotene spermatocytes and cytoplasmic lobes of late spermatids suggests a specific role of free zinc at the onset of meiosis and at spermiation.

Published
1998
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4. Differential regulation of leucine-rich primary response gene 1 (LRPR1) mRNA expression in rat testis and ovary

Author

M. Parvinen, K.E. Slegtenhorst-Eegdeman, M. Verhoef-Post, Axel P. N. Themmen, J. A. Grootegoed, and Developmental Biology

Subjects
Male, endocrine system, Embryology, medicine.medical_specialty, medicine.drug_class, Down-Regulation, Ovary, Biology, Gene product, Follicle-stimulating hormone, Internal medicine, Gene expression, Testis, Genetics, medicine, Animals, RNA, Messenger, Rats, Wistar, Spermatogenesis, Molecular Biology, Cells, Cultured, Messenger RNA, Leucine Zippers, Reproduction, Obstetrics and Gynecology, Cell Biology, Sertoli cell, Rats, DNA-Binding Proteins, Endocrinology, medicine.anatomical_structure, Reproductive Medicine, Bucladesine, Receptors, FSH, Female, Gonadotropin, Follicle Stimulating Hormone, Follicle-stimulating hormone receptor, Developmental Biology
Abstract

textabstractIn immature rat Sertoli cells, leucine-rich primary response gene 1 (LRPR1) represents a follicle stimulating hormone (FSH)-responsive gene; the function of the encoded protein is not yet known. LRPR1 mRNA expression is up-regulated very rapidly and specifically by FSH, both in cultured Sertoli cells and in vivo in regulation in more detail, in testis and ovary of fetal, immature, and adult rats. In addition, we have studied the expression of FSH receptor (FSHR) mRNA in relation to LRPR1 mRNA expression. In rat testis, LRPR1 mRNA and FSHR mRNA followed a similar expression pattern, during postnatal development and also at different stages of the spermatogenic cycle in the adult rat. Furthermore, after short-term challenge of the FSH signal transduction pathway in intact immature rats by injection with a relatively high dose of FSH, an inverse relationship between LRPR1 mRNA (up-regulation) and FSHR mRNA expression (down-regulation) was observed. Similar studies in the ovary provided completely different results. LRPR1 mRNA in the postnatal ovary is present well before expression of FSHR mRNA can be first detected. In addition, incubation of ovaries of immature rats with FSH or dibutyryl cyclic AMP (dbcAMP) did not result in up-regulation of LRPR1 mRNA expression. During fetal development, the LRPR1 mRNA expression pattern involved many more tissues, in contrast to the relatively tissue-specific expression of LRPR1 mRNA in gonads of 21 day old and adult rats. Moreover, LRPR1 mRNA expression could be detected as early as 12.5 days post-coitum, whereas FSHR mRNA is absent at this stage of fetal development. We concluded that the pronounced regulation of LRPR1 by FSH observed in the immature rat testis does not occur in the ovary. Furthermore, in the ovary LRPR1 mRNA expression does not appear to be dependent on FSH action. Finally, the LRPR1 gene product may play a general role during fetal development.

Published
1998

5. Lipopolysaccharide induced apoptosis of rat pancreatic acinar cells

Author

M. Parvinen, Timo J. Nevalainen, H. J. Peuravuori, K. M. Nyman, Veli J. O. Laine, and K. Henriksen

Subjects
Lipopolysaccharides, Male, medicine.medical_specialty, Pancreatic disease, Lipopolysaccharide, Fluoroimmunoassay, Apoptosis, Biology, Phospholipases A, Rats, Sprague-Dawley, Peritoneal cavity, chemistry.chemical_compound, Acinus, Internal medicine, Escherichia coli, medicine, Acinar cell, Animals, Fragmentation (cell biology), Pancreas, Gastroenterology, DNA, medicine.disease, Rats, Phospholipases A2, medicine.anatomical_structure, Endocrinology, chemistry, lipids (amino acids, peptides, and proteins), Research Article, DNA Damage
Abstract

BACKGROUND--Bacterial lipopolysaccharide (LPS) has been proposed to participate in the pathogenesis of pancreatic inflammatory disease. AIMS--This study investigated the role of endotoxaemia in the pathogenesis of pancreatic acinar cell injury. METHODS--Sixty eight male Spraque-Dawley rats were used in the study. Escherichia coli LPS (5 mg/kg) was injected into the peritoneal cavity of the rats. The concentration of pancreatic phospholipase A2 (PLA2) in plasma was measured and pancreatic tissue examined by histology, in situ detection of free DNA 3'-ends, and electrophoretic DNA analysis. RESULTS--The concentration of pancreatic PLA2 increased in plasma and the catalytic activity of PLA2 increased in pancreatic tissue after an LPS injection. Apoptosis in pancreatic acinar cells and fragmentation of DNA typical of apoptosis in pancreatic tissue was seen 24 hours after an LPS injection. Pancreatic acinar atrophy was seen 72 hours after the LPS injection. CONCLUSIONS--These data show that LPS causes release of pancreatic PLA2 into blood plasma, activation of PLA2 in pancreatic tissue, and apoptosis of acinar cells.

Published
1996
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6. Stage-specific expression of pituitary adenylate cyclase-activating polypeptide (PACAP) mRNA in the rat seminiferous tubules

Author

Mika Paavola, J Kononen, Markku Pelto-Huikko, M Parvinen, and T L Penttilä

Subjects
Male, endocrine system, medicine.medical_specialty, Adenylate kinase, In situ hybridization, Biology, Cyclase, Rats, Sprague-Dawley, Paracrine signalling, Endocrinology, Internal medicine, Testis, medicine, Animals, RNA, Messenger, Northern blot, Spermatogenesis, Autocrine signalling, In Situ Hybridization, Messenger RNA, Neuropeptides, Seminiferous Tubules, Blotting, Northern, Molecular biology, Epithelium, Rats, medicine.anatomical_structure, Gene Expression Regulation, Pituitary Adenylate Cyclase-Activating Polypeptide, hormones, hormone substitutes, and hormone antagonists
Abstract

We have used in situ hybridization and Northern blot analysis with oligonucleotide probe to characterize the site of pituitary adenylate cyclase-activating polypeptide (PACAP) synthesis in the rat testis. We observed strong hybridization signal in one third of the cross-sections of the seminiferous tubules, whereas some tubules were devoid of hybridization signal, thus suggesting that PACAP mRNA is expressed in a stage-specific manner. More detailed analysis showed that PACAP mRNA was present in round spermatids at stages III-VII of the cycle. Northern blot hybridization to RNAs extracted from samples of seminiferous tubules at different stages of the epithelial cycle confirmed that expression of PACAP mRNA is restricted to specific stages of the cycle. The highest amount of PACAP mRNA was detected at stages V to early -VII of the cycle, whereas very low levels of mRNA were present at stages I-II and IX-XIV. The present results demonstrate that PACAP mRNA is expressed in the developing germ cells. This suggests that PACAP may function as a paracrine or autocrine regulatory factor for the Sertoli and germ cells, with a specific function during early spermiogenesis, shortly before the onset of nuclear elongation, at the last period of haploid gene activity.

Published
1994
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7. Expression of inhibin α,βA and βB messenger ribonucleic acids in the normal human ovary and in polycystic ovarian syndrome

Author

T A Jaatinen, J Toppari, A Kaipia, M Parvinen, T Ekfors, and Tarja-Leena Penttilä

Subjects
endocrine system, medicine.medical_specialty, endocrine system diseases, Endocrinology, Diabetes and Metabolism, Gene Expression, Alpha (ethology), Ovary, Biology, Endocrinology, Internal medicine, Follicular phase, medicine, Humans, Inhibins, RNA, Messenger, Beta (finance), In Situ Hybridization, Cellular localization, G alpha subunit, Granulosa Cells, Polycystic ovary, female genital diseases and pregnancy complications, medicine.anatomical_structure, Follicular Phase, Theca, Theca Cells, Female, hormones, hormone substitutes, and hormone antagonists, Polycystic Ovary Syndrome
Abstract

We studied the cellular distribution of inhibin α, βA and βB mRNAs in the normal human ovary and in polycystic ovarian syndrome (PCOS) by in situ hybridization. Our results show that human granulosa cells express inhibin α, βA and βB subunit mRNAs, and theca cells express inhibin α and βA subunit mRNAs. The co-localization of α and βA mRNAs in theca cells supports the hypothesis that inhibin also has an autocrine function in these cells. We did not detect any inhibin subunit mRNA in the granulosa cells of atretic follicles, while theca cells also expressed α subunit mRNA in those follicles. The present findings suggest that the expression of inhibin subunits is regulated differently in human follicular granulosa and theca cells. It has been speculated that inhibin may be involved in the development of PCOS. Our results show that the cellular localization of inhibin subunit mRNAs is not disturbed in PCOS ovaries. Journal of Endocrinology (1994) 143, 127–137

Published
1994
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9. Testicular toxicity and mutagenicity of steroidal and non-steroidal estrogens in the male mouse

Author

K. Jahnukainen, R. Santti, L. Pylkkänen, and M. Parvinen

Subjects
Male, endocrine system, medicine.medical_specialty, medicine.drug_class, Injections, Subcutaneous, Diethylstilbestrol, Biology, Toxicology, Mice, chemistry.chemical_compound, Pregnancy, In vivo, Rete testis, Internal medicine, Testis, Genetics, medicine, Zeranol, Animals, Micronuclei, Chromosome-Defective, Chromosome Aberrations, Micronucleus Tests, Estradiol, urogenital system, Seminiferous Tubules, Spermatids, Spermatozoa, medicine.anatomical_structure, Endocrinology, Animals, Newborn, chemistry, Estrogen, Micronucleus test, Toxicity, Sperm Head, Female, Micronucleus, medicine.drug
Abstract

The mutagenicity and toxicity of diethylstilbestrol (DES), 17 beta-estradiol and zeranol on the male mouse germ cells were investigated with meiotic micronucleus assays in vivo and in vitro, sperm-head abnormality test and morphometry. Further, the developmental effects of DES on testicular morphology were explored. Micronucleus induction was observed at 10(-7) M concentration of DES and 17 beta-estradiol in vitro, but other treatments yielded negative results. The micronucleus assay in vivo revealed a small number of micronuclei in early haploid spermatids 17 days after a single subcutaneous injection of DES 50 mg/kg, whereas estradiol and zeranol gave negative results. The sperm-head abnormality rates were significantly elevated 5 weeks after treatments with high doses of DES, 17 beta-estradiol and zeranol, and testicular morphometry revealed transient changes in the volume densities of testicular tissue components. Prenatal and neonatal estrogen administration resulted in permanent alterations in seminiferous epithelium and dilatation of the rete testis, but did not affect micronucleus or sperm-head abnormality rates. The mutagenicity and toxicity of hormones in the mouse testis paralleled the hormonal activity of these compounds. Early estrogenization was the most sensitive toxicity test, followed by in vitro meiotic micronucleus induction, whereas the sperm-head abnormality assay and morphological analysis did not reveal subtle changes.

Published
1991
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10. Morphometric evaluations of testicular tissues from azoospermic boars in Finnish Yorkshire and Landrace breeds

Author

M. Parvinen, Juhani Taponen, C. Kopp, Antti Flyckt, R. Ijäs, and Magnus Andersson

Subjects
Male, endocrine system, Testicular tissue, Sterility, Swine, medicine.medical_treatment, Spermatocyte, Biology, Andrology, 03 medical and health sciences, 0302 clinical medicine, Food Animals, Testis, medicine, Animals, Small Animals, 030304 developmental biology, Azoospermia, Swine Diseases, 0303 health sciences, 030219 obstetrics & reproductive medicine, urogenital system, Equine, Artificial insemination, medicine.disease, Seminiferous tubule, medicine.anatomical_structure, Animal Science and Zoology, Spermatogenesis
Abstract

In 1996–2005, ejaculates of 2048 boars were collected. All boars were intended for use in artificial insemination or natural breeding and had two descended testes. Azoospermia was present in 16 of the 1097 Yorkshire boars (1.5%) and in 2 of the 951 Landrace boars (0.2%). The two most frequent diagnoses of azoospermia were arrested spermatogenesis at the pachytene spermatocyte stage ( n = 8) and segmental aplasia of the Wolffian ducts ( n = 7). Morphometric evaluations of testicular tissues of azoospermic boars were performed using an image analyzer. The morphometric evaluations revealed decreased portions and diameter of seminiferous tubule in tissue slides from the studied azoospermic boars compared with normal boars. The use of an image analyzer for morphometric evaluations of testicular tissues proved to be a good tool to characterize findings in testicular slides of azoospermic boars.

Published
2008

11. Multinuclear-multiflagellar sperm defect in a bull--a new sterilizing sperm defect

Author

C. Kopp, Antti Sukura, Ingemar Gustavsson, E Tuunainen, M. Parvinen, and Magnus Andersson

Subjects
Male, endocrine system, 040301 veterinary sciences, Spermiogenesis, medicine.medical_treatment, Cattle Diseases, Semen, Biology, Intracytoplasmic sperm injection, Male infertility, 0403 veterinary science, Andrology, 03 medical and health sciences, Sperm heteromorphism, 0302 clinical medicine, Endocrinology, Meiosis, Microscopy, Electron, Transmission, Testis, medicine, Animals, Acrosome, reproductive and urinary physiology, Infertility, Male, 030219 obstetrics & reproductive medicine, Sperm Count, urogenital system, 04 agricultural and veterinary sciences, Organ Size, medicine.disease, Sperm, Spermatozoa, Karyotyping, Sperm Tail, Mutation, Animal Science and Zoology, Cattle, Biotechnology
Abstract

The development and use of modern techniques, such as intracytoplasmic sperm injection (ICSI), gene knockout and sperm fluorescence in situ hybridization with chromosome- specific probes, have significantly increased our knowledge about sperm defects. We describe a new oligoasthenoteratozoospermic defect in a bull. Because of its morphological characteristics the defect was named the multinuclear-multiflagellar sperm defect. All spermatozoa in the ejaculate were abnormal. Many of the spermatozoa had multiple nuclei and multiple sperm tails. All spermatozoa lacked an acrosome, and only seldom did spermatozoa have a mitochondrial helix in the midpiece area. Meiosis and spermiogenesis were severely affected in this otherwise phenotypically normal bull. The sperm defects resembled the phenotype of a targeted gene knockout Hrb(-/-) (HIV-1 Rev-binding/interacting protein) mutant mouse strain, which is expressed as sterility in males, while females remain fertile. Since the father of this bull has been extensively used in at least three countries the defective gene has possibly become widespread in the red and white breeds (Ayrshire, Swedish Red and White, Norwegian Red) in the Nordic countries. However, it is not proved that the father of this bull is a carrier of this defect.

Published
2007

12. Chemical anoxia delays germ cell apoptosis in the human testis

Author

K, Erkkilä, L, Suomalainen, M, Wikström, M, Parvinen, and L, Dunkel

Subjects
Male, Antimetabolites, Prostatic Neoplasms, Apoptosis, DNA Fragmentation, Hydrogen Peroxide, Deoxyglucose, In Vitro Techniques, Middle Aged, Spermatozoa, Adenosine Monophosphate, Cell Hypoxia, Adenosine Diphosphate, Blotting, Southern, Microscopy, Electron, Adenosine Triphosphate, Oxygen Consumption, Pyruvic Acid, Testis, In Situ Nick-End Labeling, Humans, Potassium Cyanide, Glycolysis, Aged
Abstract

An understanding of testicular physiology and pathology requires knowledge of the regulation of cell death. Previous observation of suppression of apoptosis by hypoxia suggested a role for ATP in germ cell death. However, the exact effects of ATP production on germ cell death and of apoptosis on the levels of ATP and other adenine nucleotides (ANs) have remained unclear. We investigated the levels of ANs during human testicular apoptosis (analyzed by HPLC) and the role of chemical anoxia in germ cell death (detected by Southern blot analysis of DNA fragmentation, in situ end labeling of DNA, and electron microscopy). Incubation of seminiferous tubule segments under serum-free conditions induced apoptosis and concomitantly decreased the levels of ANs. Chemical anoxia, induced with potassium cyanide (KCN), an inhibitor of mitochondrial respiration, dropped ATP levels further and suppressed apoptosis at 4 h. After 24 h, many of the testicular cells underwent delayed apoptosis despite ATP depletion. Some cells showed signs of necrosis or toxicity. The addition of 2-deoxyglucose, an antimetabolite of glycolysis, did not alter the results obtained with KCN alone, whereas a toxic concentration of hydrogen peroxide switched apoptosis to necrosis. In most of the testicular cells, mitochondrial respiration appears to play a crucial role in controlling primary cell death cascades. In the human testis, there seem to be secondary apoptotic pathways that do not require functional respiration (or ATP).

Published
2003

13. Bleomycin, vincristine, lomustine and dacarbazine (BOLD) in combination with recombinant interferon alpha-2b for metastatic uveal melanoma

Author

Tero Kivelä, Wim H. J. Kruit, L.-M. Parvinen, O Kloke, E. Kumpulainen, Seppo Pyrhönen, Johan Hansson, M Hahka-Kemppinen, Martin Gore, Meri-Sisko Vuoristo, Yves Humblet, Stefan Suciu, and Medical Oncology

Subjects
Adult, Male, Uveal Neoplasms, Cancer Research, medicine.medical_specialty, Vincristine, medicine.medical_treatment, Dacarbazine, Alpha interferon, Interferon alpha-2, Gastroenterology, Disease-Free Survival, Bleomycin, Lomustine, Internal medicine, Antineoplastic Combined Chemotherapy Protocols, medicine, Humans, Prospective Studies, Neoplasm Metastasis, Melanoma, Aged, Chemotherapy, business.industry, Interferon-alpha, Uvea, Middle Aged, medicine.disease, Recombinant Proteins, Surgery, medicine.anatomical_structure, Treatment Outcome, Oncology, Tolerability, Feasibility Studies, Female, business, medicine.drug
Abstract

This EORTC multicentre study analysed the efficacy and tolerability in patients with metastatic uveal melanoma of BOLD chemotherapy in combination with recombinant interferon alpha-2b. The dose of bleomycin was 15 mg on days 2 and 5, of vincristine 1 mg/m(2) on days 1 and 4, of lomustine 80 mg on day 1, and of dacarbazine (DTIC) 200 mg/m(2) on days 1-5, given every 4 weeks for a minimum of two cycles. Subcutaneous (s.c.) interferon alpha-2b at a dose of 3 x 10(6) IU was initiated on day 8 of the first cycle, and continued at a dose of 6 x 10(6) IU three times per week after 6 weeks. A median of two cycles were administered to 24 patients (median age 60.5 years). None achieved an objective response (0%; 95% Confidence Interval (CI): 0-14), 2 (8.3%) remained stable, 20 showed progression, and 2 (8.3%) were invaluable. The median progression-free survival was 1.9 months (95% CI: 1.8-3.4) and overall survival 10.6 months (95% CI: 6.9-16.4). Overall survival improved with increasingly favourable pretreatment characteristics (median, 14.7 versus 6.9 versus 6.0 months for Helsinki University Central Hospital (HUCH) Working Formulation stages IVBa, IVBb and IVBc, respectively; P=0.018). Grade 3 alopecia and neurotoxicity occurred in 13% of the patients. This multicentre study did not confirm earlier reports that BOLD with human leucocyte or recombinant interferon would induce at least 15% objective responses in metastatic uveal melanoma.

Published
2003

14. Serum adhesion molecules and interleukin-2 receptor as markers of tumour load and prognosis in advanced cutaneous melanoma

Author

Merja Korpela, Heini Huhtala, Meri-Sisko Vuoristo, Pirkko-Liisa Kellokumpu-Lehtinen, M Hahka-Kemppinen, E. Kumpulainen, L.-M. Parvinen, and Seppo Laine

Subjects
Interleukin 2, Adult, Male, Cancer Research, Pathology, medicine.medical_specialty, Lung Neoplasms, Skin Neoplasms, medicine.medical_treatment, Intercellular Adhesion Molecule-1, Vascular Cell Adhesion Molecule-1, Bone Neoplasms, Biology, Disease-Free Survival, Metastasis, Antineoplastic Combined Chemotherapy Protocols, medicine, Biomarkers, Tumor, Humans, Receptor, Melanoma, Aged, Univariate analysis, Cell adhesion molecule, Liver Neoplasms, Receptors, Interleukin-2, Middle Aged, medicine.disease, Neoplasm Proteins, Cytokine, Oncology, Cutaneous melanoma, Multivariate Analysis, Cancer research, Female, medicine.drug, Follow-Up Studies
Abstract

Cell adhesion molecules are cell surface glycoproteins that may act as mediators in the metastatic process. Soluble interleukin-2 receptor (sIL-2R) is an immunological marker that may also serve as an indicator of tumour progression. Normal and neoplastic cells are capable of releasing these molecules into circulation. We evaluated the association between pretreatment serum levels of soluble intercellular adhesion molecule 1 (sICAM-1), vascular cell adhesion molecule 1 (sVCAM-1) and sIL-2R and metastases and survival in 50 patients with advanced melanoma. The patients with liver and/or bone metastases had significantly higher sICAM-1 levels than those with soft tissue and/or lung involvement ( P =0.002). In addition, there was a trend towards higher sIL-2R levels in patients with more metastatic sites ( P =0.07). In univariate analysis, the number of metastatic sites ( P =0.0001, odds ratio (OR) 3.0, 95% confidence interval (CI): 1.7–5.3), the metastatic site ( P =0.01, OR 2.3, 95% CI: 1.2–4.4) and the levels of sICAM-1 ( P =0.011, OR 2.5, 95% CI: 1.2–5.0), sVCAM-1 ( P =0.036, OR 2.1, 95% CI: 1.0–4.3) and sIL-2R ( P =0.0016, OR 3.0, 95% CI: 1.5–6.0) were found to be statistically significant prognostic factors for survival. In multivariate analysis, the number of metastatic sites was the dominant prognostic indicator. After it was excluded from the analysis, the sIL-2R level and the metastatic site were found to be significant. It can be concluded, that high sICAM-1 levels suggest liver metastases and sIL-2R seems to serve as a marker of tumour load in metastatic melanoma. Furthermore, the sIL-2R level appears to add to clinical data predicting the patient's outcome.

Published
2001

15. Evaluation of the 5'-flanking regions of murine glutathione peroxidase five and cysteine-rich secretory protein-1 genes for directing transgene expression in mouse epididymis

Author

P P, Lahti, R, Shariatmadari, J K, Penttinen, J R, Drevet, B, Haendler, M, Vierula, M, Parvinen, I T, Huhtaniemi, and M, Poutanen

Subjects
Epididymis, Male, Glutathione Peroxidase, Membrane Glycoproteins, Reverse Transcriptase Polymerase Chain Reaction, Recombinant Fusion Proteins, Green Fluorescent Proteins, Gene Expression, Mice, Transgenic, Seminiferous Tubules, Blotting, Northern, Embryo Transfer, Transfection, Luminescent Proteins, Mice, Testicular Hormones, Seminiferous Epithelium, Animals, Tissue Distribution, RNA, Messenger, Salivary Proteins and Peptides, Promoter Regions, Genetic, Spermatogenesis
Abstract

Based on strong epididymal expression of the mouse glutathione peroxidase 5 (GPX5) and cysteine-rich secretory protein-1 (CRISP-1) genes, we evaluated whether the 5.0-kilobase (kb)-long GPX5 and 3.8-kb-long CRISP-1 gene 5'-flanking regions could be used to target expression of genes of interest into the epididymis in transgenic mice. Of the two candidate promoters investigated, the CRISP-1 promoter-driven enhanced green fluorescent protein (EGFP) reporter gene was highly expressed in the tubular compartment of the testis in all stages of the seminiferous epithelial cycle between pachytene spermatocytes at stage VII to elongated spermatids at step 16. In contrast to CRISP-1, the 5.0-kb 5' region of the mouse GPX5 gene directed EGFP expression to the epididymis. In the various GPX5-EGFP mouse lines, strongest expression of EGFP mRNA was found in the epididymis, but low levels of reporter gene mRNA were detected in several other tissues. Strong EGFP fluorescence was found in the principal cells of the distal caput region of epididymis, and few fluorescent cells were also detected in the cauda region. No EGFP fluorescence was detected in the corpus region or in the other tissues analyzed. Hence, it is evident that the 5.0-kb 5'-flanking region of GPX5 promoter is suitable for directing the expression of structural genes of interest into the caput epididymidis in transgenic mice.

Published
2001

16. Stage-specific inhibition of deoxyribonucleic acid synthesis and induction of apoptosis by antracyclines in cultured rat spermatogenic cells

Author

K, Jahnukainen, M, Hou, M, Parvinen, S, Eksborg, and O, Söder

Subjects
Male, Antibiotics, Antineoplastic, Mitosis, Apoptosis, DNA, Seminiferous Tubules, Rats, S Phase, Rats, Sprague-Dawley, Meiosis, Doxorubicin, Animals, Idarubicin, Spermatogenesis, Cells, Cultured
Abstract

A rapid in vitro method has been developed to detect early effects of cytostatic drugs on rat spermatogenesis. The induction of programmed cell death (apoptosis) and changes in DNA synthesis induced by doxorubicin and idarubicin were measured in specific stages of the cycle of seminiferous epithelium including mitotic (stage V) and meiotic (stage VIII-IX) S-phase cells. The model was used to investigate the protective effect of an organic thiophosphate, amifostine, against the toxicity of antracyclines. Premitotic DNA synthesis was found to be more sensitive than premeiotic DNA synthesis to antracyclines. Idarubicin was more toxic than doxorubicin to germ cells in inducing apoptosis and suppressing DNA synthesis. Amifostine had no protective effect against doxorubicin- or idarubicin-induced inhibition of DNA synthesis. In contrast, a significant stimulation of DNA synthesis in premitotic cells by amifostine was found, suggesting that this compound may have a stimulative effect on spermatogenic stem cells. These data show that stage-specific dissection of the seminiferous tubules and their in vitro exposure to predetermined doses of drugs may give us a unique possibility to detect drug action and protection against the cytotoxicity of antineoplastic agents at the cellular level of the spermatogenic cycle.

Published
2000

17. Neurturin, RET, GFRalpha-1 and GFRalpha-2, but not GFRalpha-3, mRNA are expressed in mice gonads

Author

J, Widenfalk, M, Parvinen, E, Lindqvist, and L, Olson

Subjects
Epididymis, Male, Mice, Inbred BALB C, Glial Cell Line-Derived Neurotrophic Factor Receptors, Membrane Glycoproteins, Neurturin, Ovary, Proto-Oncogene Proteins c-ret, Uterus, Gene Expression, Receptor Protein-Tyrosine Kinases, Receptors, Cell Surface, Oviducts, Receptors, Nerve Growth Factor, Mice, Proto-Oncogene Proteins, Animals, Drosophila Proteins, Female, Nerve Growth Factors, RNA, Messenger, In Situ Hybridization
Abstract

The gonads are known to produce numerous hormones and also neurotrophins and their receptors. Here we demonstrate expression of glial-cell-line-derived neurotrophic factor (GDNF) family ligands and related receptors in adult mice gonads by in situ hybridization. GDNF mRNA was expressed in the ovary, but was not detectable in testis. Neurturin (NTN), another ligand in this family, gave rise to strong mRNA hybridization signals in a mosaic pattern in the seminiferous tubules of the testis at stages IX-XII and I-II of the cycle. NTN mRNA signals were also found in uterus and the oviduct. In testis, the transducing receptor RET as well as GDNF receptor alpha-1 (GFR)alpha-1 and GFRalpha-2 were distributed in complementary and overlapping patterns, the former at stages XI-XII-I and the latter at stages VII and VIII. GFRalpha-3 could not be detected. Expression of these trophic molecules suggests involvement of GDNF family ligands and related receptor components in reproduction.

Published
2000

18. Acute doxorubicin cardiotoxicity involves cardiomyocyte apoptosis

Author

O J, Arola, A, Saraste, K, Pulkki, M, Kallajoki, M, Parvinen, and L M, Voipio-Pulkki

Subjects
Male, Time Factors, Dose-Response Relationship, Drug, Doxorubicin, Myocardium, In Situ Nick-End Labeling, Animals, Apoptosis, Heart, Rats, Wistar, Rats
Abstract

Despite well-documented cardiotoxic effects, doxorubicin remains a major anticancer agent. To study the role of myocardial apoptosis following doxorubicin administration, male Wistar rats were exposed to 1.25, 2.5, and 5 mg/kg of i.p. doxorubicin and terminated on days 1-7 in groups of five. Doxorubicin caused a significant (P0.001) and dose-dependent induction of cardiomyocyte apoptosis at 24-48 h after the injection. Repeated injections of 2.5 mg/kg given every other day resulted in peaks of apoptosis at 24 h after each injection. However, no additive effect of repeated dosing was noted. In histological samples, alterations in the cytoskeletal apparatus with focal loss of contractile elements were seen after a single injection. Myocyte necrosis was absent. Thus, acute doxorubicin-induced cardiotoxicity involves cardiomyocyte apoptosis, a potentially preventable form of myocardial tissue loss.

Published
2000

20. Partial oxygen pressure and mitochondrial permeability transition affect germ cell apoptosis in the human testis

Author

K, Erkkilä, V, Pentikäinen, M, Wikström, M, Parvinen, and L, Dunkel

Subjects
Aged, 80 and over, Male, Cell Membrane Permeability, Cell Survival, Partial Pressure, Apoptosis, DNA Fragmentation, Middle Aged, Spermatids, Spermatozoa, Mitochondria, Oxygen, Blotting, Southern, Microscopy, Electron, Seminiferous Epithelium, Culture Techniques, Cyclosporine, Humans, Aged
Abstract

During regular spermatogenesis, a number of testicular germ cells degenerate by an apoptotic process that is under hormonal control. Oxidative and mitochondrial changes have been proposed to play a role in apoptosis of many cell types. Previously, whether human germ cell survival is controlled by oxygen or by effectors of the mitochondrial permeability transition has not been investigated. In the present study, apoptosis was induced in human testicular germ cells by incubating segments of seminiferous tubules without survival factors (i.e. serum or hormones; 21% oxygen). Apoptosis was significantly suppressed in an inversely dose-dependent fashion at partial oxygen pressures below 10%, as detected by Southern blot analysis of DNA fragmentation, DNA labeling in situ, and electron microscopy. Cyclosporin A and its nonimmunosuppressive derivative N-methyl-Val4-cyclosporin A prevented cell death, suggesting a key role for the mitochondrial permeability transition in apoptosis. Apoptotic cells were identified as mainly spermatocytes and spermatids, the mitochondria of which underwent morphological changes during the apoptotic process. The present results imply that to improve germ cell viability in in vitro fertilization techniques, the partial oxygen pressure should be lowered.

Published
1999

21. Cardiomyocyte apoptosis and progression of heart failure to transplantation

Author

A, Saraste, K, Pulkki, M, Kallajoki, P, Heikkilä, P, Laine, S, Mattila, M S, Nieminen, M, Parvinen, and L M, Voipio-Pulkki

Subjects
Adult, Aged, 80 and over, Cardiomyopathy, Dilated, Heart Failure, Time Factors, Myocardium, Myocardial Ischemia, Apoptosis, Middle Aged, Immunohistochemistry, Proto-Oncogene Proteins c-bcl-2, Disease Progression, In Situ Nick-End Labeling, Heart Transplantation, Humans, Aged
Abstract

Cardiomyocyte apoptosis has been found in congestive heart failure, but its clinical significance has been difficult to study. We compared the occurrence of cardiomyocyte apoptosis in explanted hearts with the progression of severe heart failure until the need for transplantation.Using the TUNEL assay, apoptotic cardiomyocytes were quantified in explanted failing hearts from patients with either idiopathic dilated cardiomyopathy (n = 21) or ischaemic heart disease (n = 14). The percentage was compared with the clinical severity and progression of endstage heart failure. Samples obtained at autopsy and during open heart surgery served as controls.The number of apoptotic cardiomyocytes was significantly increased in failing hearts regardless of aetiology (medians 0.075% in ischaemic heart disease and 0.119% in dilated cardiomyopathy) compared with control myocardium. In patients with dilated cardiomyopathy, apoptotic cardiomyocytes were more numerous in subjects with a rapidly deteriorating clinical course (0.192%, n = 10) than in patients with intermediate (0.093%, n = 6, P = 0.03) or slow (0.026%, n = 5, P = 0.003) progression. No such association was observed in patients with ischaemic heart disease, in whom we found significantly increased cardiomyocyte apoptosis adjacent to scars of previous infarctions (0.576%) in contrast to the diffuse distribution seen in dilated cardiomyopathy. Expression of Bcl-2, an antiapoptotic protein, was increased in all failing hearts by immunohistochemistry.Cardiomyocyte apoptosis is a consistent feature of end-stage heart failure in man and appears to be quantitatively related to the clinical severity of deterioration in dilated cardiomyopathy. Increased expression of Bcl-2 in cardiomyocytes indicates activation of an antiapoptotic response. These observations suggest that cardiomyocyte apoptosis is a clinically relevant and potentially modifiable pathophysiological phenomenon in severe heart failure.

Published
1999

22. Function of stem cell factor as a survival factor of spermatogonia and localization of messenger ribonucleic acid in the rat seminiferous epithelium

Author

H, Hakovirta, W, Yan, M, Kaleva, F, Zhang, K, Vänttinen, P L, Morris, M, Söder, M, Parvinen, and J, Toppari

Subjects
Male, Stem Cell Factor, Cell Survival, Gene Expression Regulation, Developmental, DNA, Blotting, Northern, Spermatogonia, Rats, Rats, Sprague-Dawley, Mice, Seminiferous Epithelium, Paracrine Communication, Animals, RNA, Messenger, Cells, Cultured
Abstract

To address the possibility that stem cell factor (SCF) is a paracrine regulator of germ cell development in the adult rat testis, stage-specific distribution of SCF messenger RNA (mRNA) was investigated with Northern blot and in situ hybridization analyses. The highest levels of SCF mRNA were found in stages II-VI of the rat seminiferous epithelial cycle, whereas the lowest levels were in stages VII-VIII. Intermediate levels of SCF mRNA were detected in stages IX-XIV-I of the cycle. The expression of the SCF gene was found to be developmentally regulated, and the expression pattern followed the process of Sertoli cell proliferation and differentiation during postnatal life. The effect of mouse recombinant SCF on spermatogonial DNA synthesis was studied using an in vitro tissue culture system for stage-defined seminiferous tubules. A significant increase in DNA synthesis in spermatogonia could be detected when tubule segments from stage XII were cultured in the presence of 100 ng/ml SCF for 48 h (P0.05) and 72 h (P0.01). This observation was further confirmed with autoradiographic analyses; almost a 100-fold increase in thymidine incorporation in the SCF-treated (100 ng/ml) tubule segments was observed compared with that in untreated samples. The results of the present study suggest that SCF is a Sertoli cell-produced paracrine regulator and acts as a survival factor for spermatogonia in the adult rat seminiferous epithelium in a stage-specific manner.

Published
1999

23. Elevated expression of lanosterol 14alpha-demethylase (CYP51) and the synthesis of oocyte meiosis-activating sterols in postmeiotic germ cells of male rats

Author

M, Strömstedt, M R, Waterman, T B, Haugen, K, Taskén, M, Parvinen, and D, Rozman

Subjects
Male, L-Lactate Dehydrogenase, Gene Expression, Spermatozoa, Rats, Meiosis, Sterol 14-Demethylase, Sterols, Farnesyl-Diphosphate Farnesyltransferase, Cytochrome P-450 Enzyme System, Testis, Oocytes, Animals, Humans, Tissue Distribution, RNA, Messenger, Oxidoreductases
Abstract

Mammalian CYP51 encodes lanosterol 14alpha-demethylase (P45014DM) that is involved in the postsqualene part of cholesterol biosynthesis. This enzyme removes the 14alpha-methyl group from lanosterol and 24,25-dihydrolanosterol producing intermediates in cholesterol biosynthesis, the oocyte meiosis-activating sterols FF-MAS and MAS-412. Human and rat CYP51 messenger RNAs (mRNAs) are expressed in all tissues, with highest levels in the testis due to the presence of an additional shorter CYP51 transcript in this tissue. In situ hybridization shows the highest CYP51 mRNA levels in seminiferous tubules, with only background levels in Leydig cells. The rat testis-specific CYP51 mRNA arises from the use of an upstream polyadenylation site and is restricted to germ cells, being most abundant in elongating spermatids in stages VII-XIV, whereas somatic CYP51 transcripts are present in all cells. In contrast, the mRNA levels of squalene synthase are maximal in round spermatids, and no germ cell-specific transcript is observed. The rat male germ cell-specific CYP51 transcript is translated in vitro to two proteins of approximately 55 and 53.5 kDa. CYP51 activity is higher in protein extracts of testes and germ cells of sexually mature rats than in prepubertal animals, in which postmeiotic germ cells are not yet present. This shows increased capacity for the production of MAS sterols by male germ cells that have already completed meiosis, suggesting that they serve a role different from meiosis activation.

Published
1998

24. Testosterone regulates apoptosis in adult human seminiferous tubules in vitro

Author

K, Erkkilä, K, Henriksén, V, Hirvonen, S, Rannikko, J, Salo, M, Parvinen, and L, Dunkel

Subjects
Adult, Aged, 80 and over, Male, Blotting, Southern, Microscopy, Electron, Culture Techniques, Humans, Apoptosis, Testosterone, DNA Fragmentation, Middle Aged, Seminiferous Tubules, Aged
Abstract

In the present study an in vitro model was developed and characterized for evaluation of the role of apoptosis in adult human testes. The samples came from adult men undergoing orchidectomy for prostate or testicular cancer. Segments of seminiferous tubules were isolated and incubated under serum-free conditions in the absence or presence of testosterone. Apoptosis was assessed by low mol wt DNA fragmentation (185-bp multiples) by use of 3'-end-labeled DNA, in situ end labeling, and morphological detection under light and electron microscopy. During the 4-h incubation, a 15-fold increase was seen in apoptotic DNA fragmentation. The extent of low mol wt DNA showed a time-dependent increase and reached a 20-fold intensity in 24 h of incubation compared to the level at 0 h. Apoptosis was significantly suppressed by testosterone concentrations of 10(-7) and 10(-6) mol/L during the first 4 h of incubation. Apoptotic cells were identified mainly as spermatocytes and occasionally as spermatids. We conclude that apoptosis is induced in human seminiferous tubules under serum-free conditions in vitro. That this apoptosis is suppressed by testosterone indicates that testosterone in the human male is a critical germ cell survival factor. The model created in the present study provides a valuable tool for further investigation of hormonal and gene regulation of human germ cell death and survival.

Published
1997

25. Stage-specific expression of the FSH receptor gene in the prepubertal and adult rat seminiferous epithelium

Author

J Toppari, Tarja-Leena Penttilä, Feng Zhang, A Rannikko, I Huhtaniemi, and M Parvinen

Subjects
Male, endocrine system, medicine.medical_specialty, Endocrinology, Diabetes and Metabolism, Population, Gene Expression, In situ hybridization, Biology, Testicle, Rats, Sprague-Dawley, Endocrinology, Spermatocytes, Internal medicine, Gene expression, medicine, Animals, RNA, Messenger, Sexual Maturation, education, Spermatogenesis, In Situ Hybridization, education.field_of_study, Sertoli Cells, Cell Cycle, Sertoli cell, Blotting, Northern, Rats, medicine.anatomical_structure, Seminiferous tubule, Seminiferous Epithelium, Receptors, FSH, Follicle-stimulating hormone receptor
Abstract

Stage-specific expression of the FSH receptor (FSHR) gene in the rat seminiferous epithelium was studied. Using transillumination-assisted microdissection for sample preparation and Northern hybridization for analysis of total RNA, we first reassessed the stage specificity of the FSHR gene expression in the adult rat testis. Sixfold higher FSHR mRNA levels were found in stages XIII–I compared with stage VI of the seminiferous epithelial cycle, which had the lowest signal level (PIn situ hybridization showed distribution of grains which confirmed the data obtained by Northern analysis. Prepubertal stage-specific FSHR gene expression was studied using in situ hybridization. Stage specificity could first be demonstrated at the age of 16 days when the average grain counts in stages I–IV were threefold higher than in stages VI–VII (P Journal of Endocrinology (1996) 151, 29–35

Published
1996

26. Stage-specific apoptosis in the rat seminiferous epithelium: quantification of irradiation effects

Author

K, Henriksén, J, Kulmala, J, Toppari, K, Mehrotra, and M, Parvinen

Subjects
Male, Microscopy, Electron, Seminiferous Epithelium, Cell Cycle, Animals, Autoradiography, Apoptosis, DNA, Radiation Dosage, Rats
Abstract

The effects of 3 Gy local X-irradiation on the adult rat testis were studied together with exact determination of the radiation dose distribution in the testis. Seminiferous tubule segments were isolated 8-66 hours postirradiation (p.i.), squashed between a microscope slide and a coverslip, and the exact stage of the seminiferous epithelial cycle was identified under a phase-contrast microscope. The squash preparations were subjected to in situ end labeling (ISEL) for visualization and quantification of apoptotic cells. In controls, the highest numbers of apoptotic cells were scored in stages XII-XIV and I. In situ end-label staining of cells was observed in A3-A4 spermatogonia, spermatocytes at zygotene, pachytene, and meiotic division phases, as well as in early spermatids. In irradiated testes, from 8 hours p.i. and onward, intermediate- and B-type spermatogonia were sensitive at stages II-VI. At 42 hours, in stage I, elevated numbers of degenerating spermatocytes were seen. Most of them had not undergone meiotic divisions at stage XIV and showed an apoptotic type of degeneration at stage I. At the time of irradiation, the cells were in stage XIII, suggesting that diakinetic spermatocytes are particularly sensitive to irradiation. Also, preleptotene-zygotene spermatocytes in stages VII-XII were sensitive to irradiation. Apoptotic-type of cell degeneration was confirmed by living cell squash preparations, electron microscopy, and DNA electrophoresis. In conclusion, irradiation may provide a useful model system for studying apoptosis, and its control in spermatogonia and meiotically dividing cells.

Published
1996

27. Variation in expression of hsp27 messenger ribonucleic acid during the cycle of the seminiferous epithelium and co-localization of hsp27 and microfilaments in Sertoli cells of the rat

Author

M J, Welsh, W, Wu, M, Parvinen, and R R, Gilmont

Subjects
Male, Sertoli Cells, Base Sequence, Blotting, Western, Molecular Sequence Data, Fluorescent Antibody Technique, Gene Expression, Actins, Rats, Rats, Sprague-Dawley, Actin Cytoskeleton, Seminiferous Epithelium, Testis, Animals, Amino Acid Sequence, RNA, Messenger, Follicle Stimulating Hormone, Spermatogenesis, Cells, Cultured, Heat-Shock Proteins
Abstract

The purpose of these studies was to define expression of hsp27 mRNA during the cycle of the seminiferous epithelium and to determine the distribution of hsp27 protein in the rat testis. To study hsp27 mRNA expression, a rat hsp27 cDNA was isolated and sequenced (GenBank no. M86389). The cDNA was used in Northern blot analysis to estimate the relative levels of hsp27 mRNA in rat seminiferous tubule segments selected for different stages of the cycle of the seminiferous epithelium. The level of hsp27 mRNA was low during stages IX-XII of the cycle of the seminiferous epithelium. Approximately 15-fold higher levels of hsp27 mRNA were expressed during stages II-VI, with intermediate levels being expressed during stages XIII-I and VII-VIII. No effect of FSH on hsp27 mRNA expression was detected in cultured Sertoli cells, suggesting that hsp27 synthesis in Sertoli cells is not directly regulated by FSH. The distribution of hsp27 was also studied by use of immunofluorescence in frozen sections of rat testis, in isolated seminiferous tubules, in primary cultures of Sertoli cells isolated from 19-26-day-old rats, in peritubular myoid cells from 26-day-old rats, and in several cell lines. Microfilaments were localized in similar preparations by using rhodamine-phalloidin or BODIPY-phallicidin (Molecular Probes, Eugene, OR). The hsp27 was co-localized with micro-filaments in Sertoli cells from 20-day-old and older rats, but not in Sertoli cells from younger rats. In other cell types, hsp27 was diffusely distributed throughout the cytoplasm. These results demonstrate that hsp27 expression varies with the cycle of the seminiferous epithelium and provide the first direct morphological evidence that hsp27 is associated with microfilaments in a normal, intact tissue. They also suggest that Sertoli cell micro-filaments, by virtue of their associated hsp27, may be different in composition and function from microfilaments of peritubular myoid cells and many other cell types.

Published
1996

28. Anti-müllerian hormone and anti-müllerian hormone type II receptor messenger ribonucleic acid expression during postnatal testis development and in the adult testis of the rat

Author

M. Parvinen, Willy M. Baarends, Jenny A. Visser, D. G. De Rooij, A. P. N. Themmen, Jos W. Hoogerbrugge, J. A. Grootegoed, and M. Post

Subjects
Anti-Mullerian Hormone, Male, endocrine system, medicine.medical_specialty, Receptors, Peptide, Mullerian Ducts, Biology, Endocrinology, Internal medicine, Cryptorchidism, Testis, medicine, Animals, RNA, Messenger, Rats, Wistar, Spermatogenesis, Glycoproteins, Messenger RNA, Sexual differentiation, urogenital system, Age Factors, Anti-Müllerian hormone, Sertoli cell, Growth Inhibitors, Rats, Testicular Hormones, medicine.anatomical_structure, biology.protein, Male sex differentiation, Receptors, Transforming Growth Factor beta, Hormone
Abstract

Anti-mullerian hormone (AMH) induces degeneration of the mullerian ducts during male sex differentiation and may have additional functions concerning gonadal development. In the immature rat testis, there is a marked developmental increase in AMH type II receptor (AMHRII) messenger RNA (mRNA) expression in Sertoli cells, concomitant with the initiation of spermatogenesis. AMHRII mRNA is also expressed at a high level in Sertoli cells in adult rats. To obtain information about the possible functions of AMH in the testis, we investigated the postnatal expression patterns of the genes encoding AMH and AMHRII in the rat testis in more detail. Using RNase protection assays, AMH and AMHRII mRNA expression was measured in total RNA preparations from testes or testicular tubule segments isolated from control rats and from rats that had received various treatments. The testicular level of AMHRII mRNA was found to be much higher than that of AMH mRNA in adult rats. AMH mRNA was detected at a maximal level at stage VII of the spermatogenic cycle and at a low level at the other stages. AMHRII mRNA increases from stage XIII, is highest at stages VI and VII, and then rapidly declines at stage VIII to almost undetectable levels at stages IX-XII. It was found that the increase in testicular AMHRII mRNA expression during the first 3 weeks of postnatal development also occurs in sterile rats (prenatally irradiated), and hence, is independent of the presence or absence of germ cells. Yet, the total testicular level of AMHRII mRNA was decreased in sterile adult rats (prenatally irradiated or experimental cryptorchidism), as compared with intact control rats. However, treatment of adult rats with methoxyacetic acid or hydroxyurea, which resulted in partial germ cell depletion, had no effect on total testicular AMHRII mRNA expression. We conclude that a combination of multiple spermatogenic cycle events, possibly involving changes of Sertoli cell structure and/or Sertoli cell-basal membrane interactions, regulate autocrine AMH action on Sertoli cells, in particular at stage VII of the spermatogenic cycle.

Published
1995

29. In-situ quantification of stage-specific apoptosis in the rat seminiferous epithelium: effects of short-term experimental cryptorchidism

Author

K, Henriksén, H, Hakovirta, and M, Parvinen

Subjects
Male, Analysis of Variance, Apoptosis, DNA, Seminiferous Tubules, Spermatids, Spermatozoa, Epithelium, Rats, Rats, Sprague-Dawley, Spermatocytes, Cryptorchidism, Animals, Microscopy, Phase-Contrast
Abstract

Two techniques have been combined for quantification of apoptotic germ cells in defined stages of the cycle of the seminiferous epithelium: the improved transillumination method and nonradioactive in-situ end-labelling of DNA (ISEL). Segments of rat seminiferous tubules were squashed between a microscope slide and coverslip, and the stage identified under a phase-contrast microscope. After fixation, apoptotic cells were detected by ISEL and scored per 1 mm tubule. In the normal testis apoptotic cells were found in all stages, the highest frequency occurring in stages XII-XIV (19 cells/mm). In short-term (24 and 48 h) experimentally cryptorchid testes, a significant increase in number of apoptotic germ cells was evident in all stages, except for VI and VIII. Apoptosis of germ cells was confirmed by electrophoresis of radioactively labelled DNA from stages VII-VIII and XIII-I. It is proposed that apoptosis is a means of eliminating the most sensitive germ cells after short-term experimental cryptorchidism.

Published
1995

30. Haploid gene expression: temporal onset and storage patterns of 13 novel transcripts during rat and mouse spermiogenesis

Author

T L, Penttilä, L, Yuan, P, Mali, C, Höög, and M, Parvinen

Subjects
Male, DNA, Complementary, Time Factors, Base Sequence, Transcription, Genetic, Molecular Sequence Data, Ribonuclease H, Gene Expression, Haploidy, Blotting, Northern, Rats, Rats, Sprague-Dawley, Mice, Germ Cells, Testis, Animals, RNA, Messenger, Poly A, Spermatogenesis, In Situ Hybridization
Abstract

The temporal and spatial expression of thirteen novel spermatid-specific genes corresponding to cDNA clones isolated from an adult mouse testis library was analyzed. Northern analysis of RNA from seminiferous tubules at defined stages of the rat and mouse seminiferous epithelial cycle and in situ hybridization of testis sections revealed that these mRNAs were expressed in a stage-specific manner. The expression of all mRNAs was first detected in early round spermatids, and it increased to abundance during stages VII-VIII of the epithelial cycle. Twelve out of thirteen mRNAs were found not only in round spermatids but also in transcriptionally inactive elongated spermatids, suggesting that they are stored and regulated at the translational level. The variation in the length of the poly(A) tail was detected for four of the transcripts, represented by cDNA clones MTEST70, MTEST627, MTEST641, and MTEST643 at defined stages of the cycle. Similarity in the stage-specific expression pattern displayed by this group of haploid-specific genes strongly suggests the presence of common regulatory mechanisms that act during spermiogenesis, and these genes also provide a means for further studies of these mechanisms.

Published
1995

31. Expression of mitochondrial heat shock protein 60 in distinct cell types and defined stages of rat seminiferous epithelium

Author

A, Meinhardt, M, Parvinen, M, Bacher, G, Aumüller, H, Hakovirta, A, Yagi, and J, Seitz

Subjects
Male, Sertoli Cells, Base Sequence, Blotting, Western, Molecular Sequence Data, Gene Expression, Leydig Cells, Chaperonin 60, Immunohistochemistry, Polymerase Chain Reaction, Spermatozoa, Mitochondria, Rats, Seminiferous Epithelium, Animals, RNA, Messenger, Microscopy, Immunoelectron, Spermatogenesis
Abstract

Changes in the level of the gene transcript of heat shock protein (hsp)60, a mitochondrial chaperonin, during the cycle of rat seminiferous epithelium and its cellular localization were studied. The seminiferous epithelium showed a cell type-specific expression of hsp60. Immunostaining of adult rat testis revealed localization in Sertoli and Leydig cells. In germ cells, mitochondria of spermatogonia and early primary spermatocytes were immunoreactive for hsp60. Mitochondria of all other germ cell types were completely negative for hsp60. Stage-specific expression of hsp60 was determined from pooled segments of stage-specific microdissected tubules by a combination of Western blotting and polymerase chain reaction (PCR). High concentrations of hsp60 were found in stages I-V and IX-XIV, and low levels were detected in the other stages, i.e., VI-VIII. In stages with high hsp60 expression, spermatogonia divide mitotically, whereas in stages lacking mitosis, the hsp60 level was much weaker. In seminiferous epithelium, two different types of mitochondria are present. Therefore, immunoelectron microscopy was used to differentiate these two morphologically distinct types of mitochondria. The crista type of mitochondria (e.g., in Sertoli cells and spermatogonia) reacted with the antibody against hsp60, whereas hsp60 was negative in so-called "condensed"-type mitochondria found in midpachytene spermatocytes and more advanced germ cells. It could be shown for the first time that expression of the hsp60 gene is regulated during the cycle of the seminiferous epithelium. The results indicate that the gene product is primarily needed during the initial steps of spermatogenesis in which most of the cell divisions occur, while its expression during the differentiation of spermatids and sperm is obviously not necessary. The presence of hsp60 in stages with mitotic activity suggests a very active mitochondrial protein import and protein assembly machinery that generates further mitochondria for the dividing cells.

Published
1995

32. Expression of the mad gene during cell differentiation in vivo and its inhibition of cell growth in vitro

Author

A Lymboussakis, Imre Vastrik, T L Penttilä, M Parvinen, Arja Kaipainen, Kari Alitalo, and Riitta Alitalo

Subjects
Male, animal structures, Cell division, Cellular differentiation, Molecular Sequence Data, Basic helix-loop-helix leucine zipper transcription factors, Biology, Cell Line, 03 medical and health sciences, Mice, 0302 clinical medicine, Testis, medicine, Animals, Humans, Neoplastic transformation, Amino Acid Sequence, RNA, Messenger, Transcription factor, 030304 developmental biology, 0303 health sciences, Cell growth, Basic Helix-Loop-Helix Leucine Zipper Transcription Factors, Brain, Cell Differentiation, Cell Biology, Articles, Molecular biology, Cell biology, Rats, DNA-Binding Proteins, Repressor Proteins, medicine.anatomical_structure, Liver, Cell culture, Organ Specificity, 030220 oncology & carcinogenesis, Mice, Inbred CBA, Keratinocyte, Sequence Alignment, Cell Division
Abstract

Mad is a basic region helix-loop-helix leucine zipper transcription factor which can dimerize with the Max protein and antagonize transcriptional activation by the Myc-Max transcription factor heterodimer. While the expression of Myc is necessary for cell proliferation, the expression of Mad is induced upon differentiation of at least some leukemia cell lines. Here, the expression of the mad gene has been explored in developing mouse tissues. During organogenesis in mouse embryos mad mRNA was predominantly expressed in the liver and in the mantle layer of the developing brain. At later stages mad expression was detected in neuroretina, epidermis, and whisker follicles, and in adult mice mad was expressed at variable levels in most organs analyzed. Interestingly, in the skin mad was highly expressed in the differentiating epidermal keratinocytes, but not in the underlying proliferating basal keratinocyte layer. Also, in the gut mad mRNA was abundant in the intestinal villi, where cells cease proliferation and differentiate, but not in the crypts, where the intestinal epithelial cells proliferate. In the testis, mad expression was associated with the completion of meiosis and early development of haploid cells. In cell culture, Mad inhibited colony formation of a mouse keratinocyte cell line and rat embryo fibroblast transformation by Myc and Ras. The pattern of mad expression in tissues and its ability to inhibit cell growth in vitro suggests that Mad can cause the cessation of cell proliferation associated with cell differentiation in vivo.

Published
1995

33. Apoptosis in testis germ cells: developmental changes in gonadotropin dependence and localization to selective tubule stages

Author

M. Parvinen, I. Furuta, Aaron J. W. Hsueh, J. S. Tapanainen, Håkan Billig, and C. Rivier

Subjects
Male, endocrine system, medicine.medical_specialty, Cell type, medicine.drug_class, Apoptosis, Biology, Chemical Fractionation, Gonadotropin-releasing hormone antagonist, Gonadotropin-Releasing Hormone, Rats, Sprague-Dawley, Endocrinology, Internal medicine, Testis, medicine, Animals, Apoptotic DNA fragmentation, DNA, Seminiferous Tubules, Sertoli cell, Spermatozoa, Rats, Seminiferous tubule, medicine.anatomical_structure, Animals, Newborn, DNA fragmentation, Gonadotropin, Gonadotropins
Abstract

Recent studies have demonstrated apoptotic DNA fragmentation in the testis of immature rats deprived of gonadotropins. However, the exact cell type undergoing apoptosis during testis development and the age differences of gonadotropin dependence of testis cell apoptosis are unclear. The present study used gel fractionation and in situ methods to quantitate developmental changes of testis cell DNA fragmentation and to localize the specific cell type affected in developing rats with and without treatment with a GnRH antagonist. Apoptotic DNA fragmentation in whole testis was measured in rats between 8-70 days of age. A gradual increase (1.8- to 2.0-fold) in testis apoptotic DNA fragmentation was seen in rats between 16-28 days of age, compared with 8-day-old animals, followed by a decrease in adult animals. To study gonadotropin dependence of testicular apoptosis, serum FSH and, to a lesser extent, LH were suppressed by treatment with a long-acting GnRH antagonist (azaline-B, 250 micrograms/kg body wt, two injections at 2-day intervals). Pretreatment with the GnRH antagonist increased apoptotic DNA fragmentation in rats between 16-32 days of age but not in younger and adult animals demonstrating an age-related change in gonadotropin dependence. To identify the exact testis cell type undergoing apoptosis, in situ analysis of DNA fragmentation was performed. In rats at 16-24 days of age, spermatocytes in selected tubules were found to have increased DNA fragmentation. In contrast, neither Leydig cells nor Sertoli cells were affected. In 32-day-old and adult animals, increased DNA fragmentation was seen in early primary spermatocytes of some tubules. Treatment with GnRH antagonist increased the number of cells with DNA fragmentation as well as percentage of tubules affected. In animals between 16-32 days of age, meiotic spermatocytes were labeled, whereas early spermatids were also labeled in 24- and 32-day-old animals. In adult animals, the level of apoptotic DNA fragmentation was not affected by GnRH antagonist treatment. However, DNA isolated from specific stages of the seminiferous tubules of adult animals showed stage-specific changes of apoptotic DNA fragmentation with 2-fold higher levels found in stages I and XII-XIV compared with stage VIII. In situ analysis of adult testis demonstrated that spermatocytes were the major cell type affected. In conclusion, the present study demonstrated that at least three factors determine the onset of apoptosis of the male germ cells: 1) the developmental stage of the animal; 2) serum levels of gonadotropins, especially FSH; and 3) specific stage of the seminiferous epithelial cycle. The present approach provides the basis for future analysis of the role of gonadotropins and other factors in the regulation of testis cell degeneration in normal and pathological states.

Published
1995

34. Delayed diagnosis and large size of breast cancer after a false negative mammogram

Author

Kaija Holli, E. Kumpulainen, L.-M. Parvinen, H. Joensuu, V. Nikkanen, and R. Asola

Subjects
Cancer Research, medicine.medical_specialty, Time Factors, Mammary gland, Breast Neoplasms, Delayed diagnosis, Sensitivity and Specificity, Breast cancer, medicine, Axillary nodes, Mammography, Humans, Prospective Studies, Stage (cooking), False Negative Reactions, Neoplasm Staging, Gynecology, medicine.diagnostic_test, Obstetrics, business.industry, Age Factors, Middle Aged, medicine.disease, medicine.anatomical_structure, Oncology, Tumour size, Female, business, Large size
Abstract

The aim of this prospective, multicentre study was to investigate the effects of a false negative mammogram on treatment delay and tumour size. Among 306 consecutive women with histologically diagnosed, invasive breast cancer, the frequency of a false negative mammogram was small (13%) among women aged over 50 years, but 35% among those aged 50 or younger (P < 0.0001). Forty-five per cent of the women with a false negative mammogram had a longer than 2-month and 29% a longer than 6-month interval from mammography to surgery as compared with only 2 and 0% of women, respectively, who had a true positive mammogram (P < 0.0001 for both). Women with a false negative mammogram and a longer than 2-month interval to surgery had larger primary tumour size (60 versus 26% pT2-4, P = 0.005) and more often positive axillary nodes (60% versus 32% pN+, P = 0.03) at the time of surgery than those with a shorter delay. We conclude that a false negative mammogram is common in women younger than 50, and may lead to treatment delay and advanced clinical stage.

Published
1994

35. Comparison of effects of 0.5 and 3.0 Gy X-irradiation on lipid peroxidation and antioxidant enzyme function in rat testis and liver

Author

V, Peltola, M, Parvinen, I, Huhtaniemi, J, Kulmala, and M, Ahotupa

Subjects
Male, Rats, Sprague-Dawley, Glutathione Peroxidase, Time Factors, Liver, Superoxide Dismutase, Testis, Animals, Lipid Peroxidation, Organ Size, Thiobarbituric Acid Reactive Substances, Glutathione Transferase, Rats
Abstract

The prooxidant effect of X-irradiation on rat testis and liver tissue was studied with doses of 0.5 and 3.0 Gy; the latter dose kills the proliferating spermatogonia and causes a maturation-depletion process in the germ cells. The level of lipid peroxidation, measured by the formation of diene conjugates and thiobarbituric acid-reactive substances (TBARS) and the activities of the antioxidant enzymes were determined 0.5 hours, 1 day, 7 days, and 31 days after the exposure. In the liver, increased levels of diene conjugation (+36%, P0.05) in the group of 3.0 Gy at 0.5 hours indicated increased lipid peroxidation. At the same time, TBARS were increased (+25%, P0.05) in the group of 0.5 Gy, but not in the 3.0-Gy group. In the testis, diene conjugation was not determined at 0.5 hours postirradiation, and at day 1 it was at the control level. The level of TBARS in the testis was below control (-11%, P0.01) in the 3.0-Gy group at day 1. At day 31 after 3.0 Gy in the testis, an increase in the amount of conjugated dienes (+24%, P0.01) was observed in parallel with a decreased level of TBARS (-15%, P0.01). The activity of superoxide dismutase (SOD) was decreased in the testis at 0.5 hours postirradiation (-28%, P0.05, and -29%, P0.05, in the groups of 0.5 and 3.0 Gy), whereafter it returned to normal by day 7. In the liver, such inactivation of SOD was not observed.(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1993

36. Identification, ontogeny, and regulation of an interleukin-6-like factor in the rat seminiferous tubule

Author

C W Bardin, V. Syed, A Kaipia, Nadine Gérard, M Parvinen, Bernard Jégou, Institut National de la Santé et de la Recherche Médicale (INSERM), Population Council, and University of Turku

Subjects
Lipopolysaccharides, Male, Aging, endocrine system, medicine.medical_specialty, Cell type, [SDV.OT]Life Sciences [q-bio]/Other [q-bio.OT], medicine.medical_treatment, 030209 endocrinology & metabolism, Testicle, Biology, Rats, Sprague-Dawley, 03 medical and health sciences, 0302 clinical medicine, Endocrinology, Internal medicine, medicine, Animals, Cells, Cultured, ComputingMilieux_MISCELLANEOUS, 030304 developmental biology, Latex beads, 0303 health sciences, Sertoli Cells, Interleukin-6, urogenital system, Monocyte, Seminiferous Tubules, Sertoli cell, Spermatids, Spermatozoa, Microspheres, Rats, Seminiferous Epithelium, Seminiferous tubule, medicine.anatomical_structure, Cytokine, Bucladesine, Follicle Stimulating Hormone, Spermatogenesis
Abstract

The present study's aims are to search for the presence of interleukin-6 bioactivity (IL-6) in medium conditioned by various testicular cell types and to investigate the cellular and hormonal regulation of testicular IL-6 production. Sertoli cells prepared from rats of increasing ages (20, 35, and 45 days) secreted IL-6 in vitro, whereas medium conditioned by pachytene spermatocytes, early spermatids, and peritubular cells showed no activity. Lipopolysaccharide (LPS) and latex beads, two known stimulators of monocyte/macrophage IL-6 production, markedly stimulated IL-6 secretion by Sertoli cells at all the ages investigated. Maximum levels of IL-6 were reached after 6 h of culture of Sertoli cells with LPS and after 24 h with latex beads. When Sertoli cells were cocultured with pachytene spermatocytes, early spermatids, or fractions containing residual bodies and cytoplasts from elongated spermatids, only the latter significantly stimulated IL-6 levels. Maximum levels of IL-6 were attained by adding 2 x 10(6) residual bodies to Sertoli cells; a significant increase in IL-6 secretion was seen after 6 h, and maximum levels were observed after 24 h. The levels of IL-6 varied throughout different stages of the seminiferous epithelium cycle; highest levels were observed in stages II-VI and lowest in stages VII-VIII. IL-6 bioactivities induced by LPS and residual bodies and cytoplasts from elongated spermatids could be totally neutralized with a specific monoclonal antibody at all of the ages studied. FSH, phorbol myristate acetate, and IL-1 alpha augmented Sertoli cell IL-6 secretion in a dose-dependent manner. Furthermore, FSH and (Bu)2cAMP differentially stimulated IL-6 secretion during the seminiferous epithelial cycle. It is concluded that the release of IL-6 from Sertoli cells is regulated by a complex interplay between residual bodies and humoral factors.

Published
1993
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37. Beta-nerve growth factor influences the expression of androgen-binding protein messenger ribonucleic acid in the rat testis

Author

P, Lönnerberg, O, Söder, M, Parvinen, E M, Ritzén, and H, Persson

Subjects
Male, Seminiferous Epithelium, Base Sequence, Molecular Sequence Data, Testis, Animals, Gene Expression, Rats, Inbred Strains, Nerve Growth Factors, RNA, Messenger, Blotting, Northern, Androgen-Binding Protein, Rats
Abstract

The effect of infusion of nerve growth factor (NGF) into the rat testis on the expression of androgen-binding protein (ABP) mRNA was studied. A major 1.7-kb and a minor 3.7-kb ABP mRNA were present at all stages of the seminiferous epithelium with maximal levels at stages VIII-XI and the lowest levels at stages IV-VI. Infusion of 15 ng/h of NGF with a mini-osmotic pump for 14 days resulted in a 2-fold increase of ABP mRNA as revealed by Northern blots, whereas the mRNA level of another Sertoli cell protein, urokinase-type plasminogen activator, remained unchanged. Image analysis of autoradiograms obtained by in situ hybridization of sections from treated testes showed a similar increase in APB mRNA compared to noninfused or PBS-infused testes. However, at the cellular level the labeling intensity for ABP mRNA over Sertoli cells of different stages of the seminiferous epithelium was the same in NGF-infused and control testes. This suggests that the increase of ABP mRNA in NGF-infused testes was caused by prolongation of stages VII-VIII with maximal ABP mRNA expression; the suggestion is supported by an increase of 30 percent in frequency of these stages in histological sections from NGF-infused testes.

Published
1992

38. Stage- and cell-specific expression of cyclic adenosine 3',5'-monophosphate-dependent protein kinases in rat seminiferous epithelium

Author

P, Lönnerberg, M, Parvinen, T, Jahnsen, V, Hansson, and H, Persson

Subjects
Male, Seminiferous Epithelium, Testis, Cyclic AMP, Animals, Gene Expression, Nucleic Acid Hybridization, Rats, Inbred Strains, RNA, Messenger, Blotting, Northern, DNA Probes, Protein Kinases, Rats
Abstract

Expression of mRNAs in the rat testis encoding cyclic AMP (cAMP)-dependent protein kinases (PKAs) was studied. A microdissection method was used to isolate 10 pools of seminiferous tubules representing various stages of the cycle of the seminiferous epithelium in combination with Northern blots and in situ hybridization. The results showed a differential expression of the four isoforms of the regulatory subunits (PKA-R) at various stages of the cycle. RI alpha mRNA was detected at approximately the same levels at all stages while expression of RI beta mRNA was low at stages XIII-III, started to increase at stages IV-V, and reached a maximum at stages VIII-XI. The level of RII alpha mRNA was low at stages II-VI, increased markedly at stage VIIa,b, and reached maximal levels at stages VIIc,d and VIII, followed by a reduced expression at later stages, RII beta mRNA levels increased significantly at stage VI with maximal levels at stages VII and VIII. In situ hybridization of sections from the adult rat testis revealed RI alpha mRNA in the layers of pachytene spermatocytes and round spermatids of all stages. RI beta mRNA was detected over late pachytene spermatocytes and round spermatids of stages VII-XIII. RII alpha mRNA was seen in the layers of round spermatids of stages VII-VIII and elongating spermatids of later stages while RII beta mRNA was detected only in the round spermatid region of stages VII-VIII and in some tubules of stages I-VI. These data show that mRNAs encoding PKA-R are expressed in a stage-specific manner in differentiating male germ cells with different patterns of expression for each subunit; this suggests specific roles for these protein kinases at different times of spermatogenesis.

Published
1992

39. Basal and FSH-stimulated steady state levels of SGP-2, alpha 2-macroglobulin, and testibumin in culture media of rat seminiferous tubules at defined stages of the epithelial cycle

Author

M, Kangasniemi, C Y, Cheng, J, Toppari, J, Grima, M, Stahler, C W, Bardin, and M, Parvinen

Subjects
Male, Clusterin, Animals, Proteins, Rats, Inbred Strains, alpha-Macroglobulins, Follicle Stimulating Hormone, Seminiferous Tubules, Spermatogenesis, Saposins, Glycoproteins, Molecular Chaperones, Rats
Abstract

Production of several proteins by rat Sertoli cells is dependent on the stage of the cycle of the seminiferous epithelium. The authors have determined steady state levels and follicle-stimulating hormone responsiveness of three Sertoli cell products in culture media of rat seminiferous tubule segments at different stages of the epithelial cycle: SGP-2 (sulfated glycoprotein-2), alpha 2-macroglobulin, and testibumin. Basal SGP-2 levels were twofold higher in stages VII through VIII compared with stages XIII to I to VI (P less than 0.05). Highest basal alpha 2-macroglobulin levels were found in stages II through VIII; this was about 35% greater than in stages XIII through I of the cycle (P less than 0.05). Basal testibumin levels were twofold higher in stages II through VI compared with stages IX through XII of the cycle. Follicle-stimulating hormone had no effect on SGP-2, but by contrast it (50 mg/L) increased the level of alpha 2-macroglobulin significantly (P less than 0.05) in stages XIII through I. Follicle-stimulating hormone treatment (10 mg/L) elevated testibumin levels at each stage-pool by about 40% (P less than 0.05). The current results using staged tubular segments in vitro demonstrate cyclic basal steady-state levels of the three proteins along the seminiferous tubules and follicle-stimulating hormone regulation of alpha 2-macroglobulin and testibumin.

Published
1992

40. In vitro stimulation of stage-specific deoxyribonucleic acid synthesis in rat seminiferous tubule segments by interleukin-1 alpha

Author

M, Parvinen, O, Söder, P, Mali, B, Fröysa, and E M, Ritzén

Subjects
DNA Replication, Male, Cell Cycle, Epithelial Cells, Rats, Inbred Strains, In Vitro Techniques, Seminiferous Tubules, Tritium, Epithelium, Recombinant Proteins, Rats, S Phase, Animals, Autoradiography, Spermatogenesis, Interleukin-1, Thymidine
Abstract

Levels of rat testicular interleukin-1-like factor (tIL-1) have been shown to correlate with DNA synthetic activity during the cycle of the rat seminiferous epithelium, suggesting its role as a spermatogonial or meiotic growth factor. To explore this further, a new in vitro model system was developed. Rat seminiferous tubule segments from stages I, V, VIIa, and VIII-IX of the cycle were isolated by transillumination-assisted microdissection, cultured in chemically defined serum-free medium supplemented with human recombinant IL-1 alpha, and labeled with [3H]thymidine. During incubation, spontaneous progression of spermatogenesis was noted. Inactive stage VIIa tubule segments differentiated to stage VIII and initiated DNA synthesis, and concomitantly started to secrete IL-1-like factor. DNA synthesis of stages VIII-IX ceased through differentiation of spermatocytes to leptotene-zygotene (stages XII-XIII of the cycle). IL-1 alpha stimulated DNA synthesis significantly in spermatogonia of stage I. Meiotic DNA synthesis at stage VIIa was stimulated (48 h/34 C) and maintained at stages VIII-IX (48 h/34 C). IL-1 alpha seems to act as a regulator of spermatogenic DNA synthesis in both mitotic and meiotic phases. It has mainly stimulating and maintaining effects, but it may also be inhibitory under certain conditions.

Published
1991

41. Production and secretion of an interleukin-1-like factor is stage-dependent and correlates with spermatogonial DNA synthesis in the rat seminiferous epithelium

Author

O, Söder, V, Syed, G V, Callard, J, Toppari, P, Pöllänen, M, Parvinen, B, Fröysa, and E M, Ritzén

Subjects
Male, Mice, Animals, Rats, Inbred Strains, DNA, Seminiferous Tubules, Spermatogenesis, Epithelium, Interleukin-1, Rats
Abstract

It has been shown previously that the intact adult rat testis produces large amounts of an interleukin-1 (IL-1)-like growth factor. The present study has investigated whether this testicular IL-1-like factor (tIL-1) is produced and secreted differentially by the fourteen stages of the seminiferous epithelial cycle in the rat testis. Seminiferous tubule segments representing defined stages were identified by transillumination-assisted microscopy and isolated by microdissection. Pooled segments were either homogenized and extracted with aqueous buffer or incubated for 24 h to produce conditioned media (CM). The recovered material was then analysed for IL-1 bioactivity in a sensitive murine thymocyte proliferation assay. When divided into four stage groups, extracts of stages II-VI, IX-XII and XIII-I showed equally high IL-1 activity whereas stage group VII-VIII showed much lower activity. More detailed analysis with 10 different stage groups showed that tIL-1 activity was undetectable in extracts of substages VIIab and VIIcd. The same pattern was seen when CM from cultured tubular segments were analysed. Labelling of seminiferous tubules with tritiated thymidine in vitro and analysis by autoradiography revealed that DNA-synthesizing spermatogonia were absent in substages VIIb and VIIc and sparse in substages VIIa and VIId. The results show that tIL-1 activity is produced in a stage-dependent manner and suggest that tIL-1 might be involved in the regulation of spermatogonial proliferation in vivo.

Published
1991

42. Local regulation of seminiferous epithelium: the role of cytokines

Author

M, Parvinen, M, Kangasniemi, A, Kaipia, P, Mali, O, Soder, P, Pollanen, J, Toppari, I, Huhtaniemi, and E M, Ritzen

Subjects
Male, Seminiferous Epithelium, Cell Cycle, Cyclic AMP, Animals, DNA, Thymus Gland, Follicle Stimulating Hormone, Spermatids, Cells, Cultured, Interleukin-1
Published
1991

43. 838 Randomised trial of dacarbazine versus BOLD chemotherapy combined with natural or recombinant alfa-interferon in patients with advanced melanoma

Author

Merja Korpela, L.-M. Parvinen, P-L Kellokumpu-Lehtinen, M. Hahka-Kemppinen, M.-S. Vuoristo, H. Seppä, and S. Pyrhönen

Subjects
Oncology, Cancer Research, medicine.medical_specialty, Chemotherapy, business.industry, medicine.medical_treatment, Dacarbazine, law.invention, law, Interferon, Internal medicine, Recombinant DNA, medicine, In patient, business, Advanced melanoma, medicine.drug
Published
2003
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45. Active movements of the chromatoid body. A possible transport mechanism for haploid gene products

Author

L M Parvinen and M Parvinen

Subjects
Male, Time Factors, Nuclear Envelope, Movement, Motion Pictures, RNA transport, Biology, symbols.namesake, Organelle, Animals, Nuclear pore, Spermatogenesis, Gene, Genetics, RNA, Articles, Cell Biology, Golgi apparatus, Spermatids, Spermatozoa, Rats, Cell biology, Organoids, symbols, Chromatoid body
Abstract

Recent data indicate that the chromatoid body typical of rat spermatogenesis may contain RNA synthesized in early spermatids by the haploid genome. Analyses of living step-1 and step-3 spermatids by time-lapse cinephotomicrography have shown that the chromatoid body moves in relation to the nuclear envelope in two different ways. Predominantly in step 1, the chromatoid body moves along the nuclear envelope on a wide area surrounding the Golgi complex and has frequent transient contacts with the latter organelle. In step 3, the chromatoid body was shown to move perpendicular to the nuclear envelope. It was seen located very transiently at the top of prominent outpocketings of the nuclear envelope with apparent material continuities through nuclear pore complexes to intranuclear particles. The rapid movements of the chromatoid body are suggested to play a role in the transport of haploid gene products in the early spermatids, including probably nucleocytoplasmic RNA transport.

Published
1979
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46. PARACRINE REGULATION OF SPERMATOGENESIS BY GROWTH FACTORS

Author

Aida Wahab, M Parvinen, and Olof Söder

Subjects
medicine.medical_specialty, Recombinant Epidermal Growth Factor, DNA synthesis, Growth factor, medicine.medical_treatment, Biology, Cell biology, Paracrine signalling, Germ cell proliferation, Endocrinology, Nerve growth factor, Internal medicine, Pediatrics, Perinatology and Child Health, medicine, Spermatogenesis, Mitosis
Abstract

We have established a testis tissue culture model which enables studies of the effects of growth factors on germ cell proliferation in vitro. Segments of seminiferous tubules of adult rat testes representing defined stages of the seminiferous epithelial cycle with representative premitotic and premeiotic germ cells were identified by transillumination and prepared by microdissection. The tubule segments were incubated at 34°and 37°C for 24, 48, and 72 h with and without growth factors and the DNA synthesis was determined at the end of the incubation. Recombinant epidermal growth factor (EGF) was found to stimulate premeiotic DNA synthesis in a dose-dependent fashion whereas premitotic DNA synthesis was only slightly affected. This indicates that EGF is mainly a meitotic growth factor during spermatogenesis. Together with previous results demonstrating specific effects of interleukin-1α, nerve growth factor and insulin-like growth factors, the present finding form the basis of a hypothesis that mitotic and meiotic proliferation of germ cells is differentially regulated by locally produced growth factors acting in a paracrine fashion.

Published
1993
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47. STAGE-DEPENDENT SERTOLI CELL FUNCTIONS

Author

M Parvinen

Subjects
medicine.medical_specialty, Endocrinology, medicine.anatomical_structure, Endocrinology, Diabetes and Metabolism, Internal medicine, medicine, General Medicine, Biology, Stage (cooking), Sertoli cell, Cell biology, Blood–testis barrier
Published
1983
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48. Stage Dependent Variation in Mn2+−-Sensitive Adenylyl Cyclase (AC) Activity in Spermatids and FSH-Sensitive AC in Sertoli Cells

Author

M. Parvinen, Jan O. Gordeladze, O. P. F. Clausen, and Vidar Hansson

Subjects
Male, endocrine system, Biology, Epithelium, Adenylyl cyclase, Follicle-stimulating hormone, chemistry.chemical_compound, Endocrinology, medicine, Animals, Manganese, Sertoli Cells, Spermatid, urogenital system, Rats, Inbred Strains, Seminiferous Tubules, Sertoli cell, Spermatids, Spermatozoa, Minimal activity, Rats, Cell biology, medicine.anatomical_structure, chemistry, Follicle Stimulating Hormone, Ploidy, Adenylyl Cyclases, Hormone
Abstract

The variation of the specific Mn2+-dependent adenylyl cyclase (AC activity in spermatids and follicle stimulating hormone (FSH)-responsive AC activities in Sertoli cells in different stages (I-XIV) of the seminiferous epithelial cycle has been investigated. Maximal Mn2+-dependent AC activity was observed in stages II-III while minimal activity was encountered in stages VII-VIII (spermiation). FSH-responsive AC activity exhibited a pattern that coincided with that of the Mn2+-dependent AC. The stage-dependent variation in spermatid AC activity cannot be explained by altered numbers of haploid cells. This raises the question whether the Sertoli cells may regulate the spermatid AC activity. Sertoli cells in various stages are all exposed to the same concentration of circulatory hormones. Hence the stage-dependent difference in FSH-responsiveness indicates that local influences (from germ cells?) may regulate the response of the AC in Sertoli cells to FSH.

Published
1982
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49. Alveolar soft part sarcoma:A report of two cases with some histochemical and ultrastructural observations

Author

Hannu Kalimo, T. O. Ekfors, M. Parvinen, V. Rantakokko, and M. Latvala

Subjects
Cancer Research, Pathology, medicine.medical_specialty, business.industry, Anatomy, respiratory system, Histogenesis, medicine.disease, Oncology, Alveolar soft part sarcoma, Ultrastructure, Medicine, Malignant soft tissue tumors, business
Abstract

In a survey of all malignant soft tissue tumors in the extremities and limb girdles in Finland between 1960 and 1969, only one alveolar soft part sarcoma was found among 246 tumors (0.4%). Another alveolar soft part sarcoma, diagnosed in 1976, was more thoroughly studied. There was evidence that the characteristic crystals of alveolar soft part sarcoma are formed from the dense granules. Both were PASM-positive at ultrastructural level. No monoamines were detected in the cells by formaldehyde-induced fluorescence. This is a further fact to nullify the theory of the paraganglionic origin of alveolar soft part sarcoma, but the question of the histogenesis of the tumor still remains open.

Published
1979
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50. Identification of living spermatogenic cells of the mouse by transillumination-phase contrast microscopic technique for ?in situ? analyses of DNA polymerase activities

Author

N B Hecht and M Parvinen

Subjects
Male, Cell type, Histology, DNA polymerase, Cellular differentiation, DNA-Directed DNA Polymerase, Mice, Testis, medicine, Animals, Microscopy, Phase-Contrast, Spermatogenesis, Acrosome, Molecular Biology, Spermatogenic Cell, DNA synthesis, biology, Histocytochemistry, Cell Differentiation, DNA Polymerase II, Cell Biology, General Medicine, Seminiferous Tubules, DNA Polymerase I, Spermatozoa, Molecular biology, Medical Laboratory Technology, Seminiferous tubule, medicine.anatomical_structure, biology.protein, Anatomy, General Agricultural and Biological Sciences
Abstract

The stages of spermatogenesis can be identified in freshly isolated, unstained adult mouse seminiferous tubules using a transillumination method. Late acrosome- and maturation phase spermatids, arranged in bundles at stages XII-VI give rise to a spotty transillumination pattern. Before spermiation, these cells form a continuous layer on the top of the seminiferous epithelium, recognized by a strong homogeneous central light absorption in the freshly isolated seminiferous tubules at stages VII and VIII. Other stages have a pale light absorption pattern. The accurate determination of the developmental stages of the germ cells was based on the morphology of the developing acrosomic system and of the nuclei of the spermatids, as revealed by phase contrast microscopy. Using this procedure, the activity levels of DNA polymerases alpha and beta have been studied by autoradiography of squash preparations. Using endogenous templates, assay conditions that differentiate between the solubilized DNA polymerases alpha and beta in vitro, were used to distinguish between these activities in situ in different stages of mouse spermatogenesis. Except in very late spermatids shortly before spermiation, DNA polymerases alpha and beta were detectable in all cell types examined. Coinciding with the nuclear protein transitions, elongating spermatids at steps 10-12 and maturation phase spermatids at steps 13-14 showed high DNA polymerase activities. As no replication occurs in these cells, the observations support the view that both DNA polymerases alpha and beta could be involved in repair DNA synthesis.

Published
1981
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