Your search keyword '"Romijn JC"' showing total 114 results

1. Stromal inhibition of prostatic epithelial cell proliferation not mediated by transforming growth factor beta

Author

Kooistra, A, primary, van den Eijnden-van Raaij, AJM, additional, Klaij, IA, additional, Romijn, JC, additional, and Schröder, FH, additional

Published

1995

2. ARREST OF THE PROLIFERATION OF RENAL AND PROSTATE CARCINOMAS OF HUMAN-ORIGIN BY INHIBITION OF MITOCHONDRIAL PROTEIN-SYNTHESIS

Author

VANDENBOGERT, C, DONTJE, BHJ, HOLTROP, M, MELIS, TE, ROMIJN, JC, VANDONGEN, JW, and KROON, AM

Published

1986

3. Decreased sperm DNA fragmentation after surgical varicocelectomy is associated with increased pregnancy rate.

Author

Smit M, Romijn JC, Wildhagen MF, Veldhoven JL, Weber RF, and Dohle GR

Subjects

Adult, Female, Humans, Infertility, Male etiology, Infertility, Male surgery, Male, Prospective Studies, Varicocele complications, DNA Fragmentation, Pregnancy statistics & numerical data, Spermatozoa, Varicocele surgery

Abstract

Purpose: We prospectively evaluated changes in sperm chromatin structure in infertile patients before and after surgical repair of varicocele, and the impact on the pregnancy rate., Materials and Methods: Included in the study were 49 men with at least a 1-year history of infertility, a palpable varicocele and oligospermia. World Health Organization semen analysis and sperm DNA damage expressed as the DNA fragmentation index using the sperm chromatin structure assay were assessed preoperatively and postoperatively. Pregnancy (spontaneous and after assisted reproductive technique) was recorded 2 years after surgery., Results: Mean sperm count, sperm concentration and sperm progressive motility improved significantly after varicocelectomy from 18.3 × 10(6) to 44.4 × 10(6), 4.8 × 10(6)/ml to 14.3 × 10(6)/ml and 16.7% to 26.6%, respectively (p <0.001). The DNA fragmentation index decreased significantly after surgery from 35.2% to 30.2% (p = 0.019). When the definition of greater than 50% improvement in sperm concentration after varicocelectomy was applied, 31 of 49 patients (63%) responded to varicocelectomy. After varicocelectomy 37% of the couples conceived spontaneously and 24% achieved pregnancy with assisted reproductive technique. The mean postoperative DNA fragmentation index was significantly higher in couples who did not conceive spontaneously or with assisted reproductive technique (p = 0.033)., Conclusions: After varicocelectomy sperm parameters significantly improved and sperm DNA fragmentation was significantly decreased. Low DNA fragmentation index values are associated with a higher pregnancy rate (spontaneous and with assisted reproductive technique). We suggest that varicocelectomy should be considered in infertile men with palpable varicocele, abnormal semen analysis and no major female factors., (Copyright © 2013 American Urological Association Education and Research, Inc. Published by Elsevier Inc. All rights reserved.)

Published

2013

4. Fatherhood in tall men treated with high-dose sex steroids during adolescence.

Author

Hendriks AE, Boellaard WP, van Casteren NJ, Romijn JC, de Jong FH, Boot AM, and Drop SL

Subjects

Adolescent, Adult, Body Mass Index, Body Weight, Educational Status, Female, Follow-Up Studies, Humans, Male, Pregnancy, Registries, Retrospective Studies, Semen physiology, Testosterone blood, Androgens therapeutic use, Body Height, Fathers, Fertility physiology

Abstract

Background/objective: Sex steroid treatment to reduce final height of tall boys has been available since the 1950s. In women, it has been shown to interfere with fertility. In men, no such data are available. We therefore evaluated fertility and gonadal function in tall men who did or did not receive high-dose androgen treatment in adolescence., Methods: We conducted a retrospective cohort study of 116 tall men, of whom 60 had been treated. Reproductive and gonadal function was assessed by standardized interview, semen analysis, endocrine parameters, ultrasound imaging, and fatherhood. Mean age at treatment commencement was 14.2 yr, and mean follow-up was 21.2 yr., Results: Sixty-six men (36 treated and 30 untreated) had attempted to achieve fatherhood. The probability of conceiving their first pregnancy within 1 yr was similar in treated and untreated men (26 vs. 24; Breslow P=0.8). Eleven treated and 13 untreated men presented with a left-sided varicocele (P=0.5). Testicular volume, sperm quality, and serum LH, FSH, and inhibin B levels were comparable between treated and untreated men. However, treated men had significantly reduced serum T levels, adjusted for known confounders [mean (sd) 13.3 (1.8) vs. 15.2 (1.9) nmol/liter; P=0.005). In addition, testicular volume and serum inhibin B and FSH levels in treated men were significantly correlated with age at treatment commencement., Conclusion: At a mean follow-up of 21 yr after high-dose androgen treatment, we conclude that fatherhood and semen quality in tall treated men are not affected. Serum testosterone levels, however, are reduced in androgen-treated men. Future research is required to determine whether declining testosterone levels may become clinically relevant for these men as they age.

Published

2010

5. Sperm chromatin structure is associated with the quality of spermatogenesis in infertile patients.

Author

Smit M, Romijn JC, Wildhagen MF, Weber RF, and Dohle GR

Subjects

Adult, Case-Control Studies, Cross-Sectional Studies, DNA Fragmentation, Follicle Stimulating Hormone blood, Humans, Infertility, Male blood, Infertility, Male diagnosis, Inhibins blood, Male, Regression Analysis, Testosterone blood, Ultrasonography, World Health Organization, Chromatin diagnostic imaging, Infertility, Male physiopathology, Spermatogenesis physiology, Spermatozoa diagnostic imaging

Abstract

Objective: To establish the diagnostic value of sperm chromatin structure assessment for the evaluation of male factor infertility, in addition to conventional andrological workup., Design: Cross-sectional controlled study., Setting: A tertiary referral andrology clinic., Patient(s): Two hundred seventy-nine male partners of infertile couples., Intervention(s): None., Main Outcome Measure(s): The DNA fragmentation index (DFI) determined by the sperm chromatin structure assay (SCSA), semen parameters, serum levels of reproductive hormones, and World Health Organization (WHO) classification of male factor subfertility., Result(s): In all patient categories, except those including patients with hypogonadotrophic hypogonadism, sperm antibodies, or normospermia, DFI was significantly higher compared with in proven fertile controls. After classification of the quality of spermatogenesis based on mean testicular volume (<10 ml vs. >15 ml), follicle stimulating hormone (FSH; > 10 U/L vs. <5 U/L), and inhibin-B (<100 nmol/L vs. >150 nmol/L), the DFI was significantly higher in patients with poor spermatogenesis (35.9%) than in patients with normal spermatogenesis (25.9%). In a multiple regression analysis, the teratozoospermia index, sperm vitality, and FSH were significant determinants of the DFI level. Male age was associated with DFI, but leukocytospermia, body mass index, and smoking were not confounders of DFI., Conclusion(s): Impaired spermatogenesis, irrespective of the WHO classification of male factor subfertility, is generally associated with an increase of sperm DNA damage., (Copyright © 2010 American Society for Reproductive Medicine. Published by Elsevier Inc. All rights reserved.)

Published

2010

6. Sperm DNA integrity in cancer patients before and after cytotoxic treatment.

Author

Smit M, van Casteren NJ, Wildhagen MF, Romijn JC, and Dohle GR

Subjects

Hodgkin Disease drug therapy, Hodgkin Disease radiotherapy, Humans, Lymphoma, Non-Hodgkin drug therapy, Lymphoma, Non-Hodgkin radiotherapy, Male, Neoplasms, Germ Cell and Embryonal drug therapy, Neoplasms, Germ Cell and Embryonal radiotherapy, Semen Analysis, Testicular Neoplasms drug therapy, Testicular Neoplasms radiotherapy, Antineoplastic Agents adverse effects, DNA Fragmentation, Spermatozoa drug effects

Abstract

Background: We assessed sperm DNA fragmentation index (DFI) in cancer patients before and after treatment to evaluate if sperm DNA integrity is compromised by cancer itself or its treatment., Methods: In a prospective study, DFI was assessed in 127 patients diagnosed with testicular germ cell tumours (TGCT), Hodgkin's lymphoma (HL), non-Hodgkin's lymphoma (NHL) and various malignancies. The severity of cancer and tumour markers at diagnosis was recorded. Follow-up DFI after treatment was available in 52 patients who were mostly less severely affected., Results: In patients diagnosed with TGCT, HL and various malignancies, pretreatment DFI levels were not significantly different from that of proven fertile controls, but in patients with NHL an increased DFI was found. An overall significant decrease in post-treatment DFI (13.2% range 5.0-70.5) compared with pretreatment values (17.1% range 5.1-66.6) was found (P = 0.040). In TGCT patients, post-treatment DFI was significantly higher in patients who were treated with radiotherapy (16.9% range 11.5-39.9) compared with that in patients treated with chemotherapy (CT) alone (10.9% range 5.5-39.9) (P = 0.037). In HL patients, the type of treatment or number of CT cycles was not associated with DFI. Overall, post-treatment DFI in cancer patients was not significantly different from that of proven fertile controls., Conclusions: In this study, the presence of cancer does not seem to negatively affect the sperm DNA integrity in TGCT and HL patients; only NHL patients showed increased DFI at the time of diagnosis compared with healthy controls. Our results confirm previous reports that DFI decreases significantly following various anti-cancer treatments. In contrast, radiotherapy in TGCT patients is associated with an increase in DFI compared with CT treatment alone.

Published

2010

7. Gonadal dysfunction in male cancer patients before cytotoxic treatment.

Author

van Casteren NJ, Boellaard WP, Romijn JC, and Dohle GR

Subjects

Adolescent, Adult, Cryopreservation, Fertility, Gonadal Disorders complications, Gonadal Disorders pathology, Gonadal Disorders physiopathology, Humans, Infertility complications, Infertility pathology, Infertility physiopathology, Inhibins, Male, Middle Aged, Neoplasms pathology, Neoplasms, Germ Cell and Embryonal pathology, Neoplasms, Germ Cell and Embryonal physiopathology, Oligospermia etiology, Oligospermia pathology, Oligospermia physiopathology, Semen, Semen Analysis, Sperm Count, Testicular Neoplasms drug therapy, Young Adult, Neoplasms complications, Neoplasms drug therapy, Neoplasms, Germ Cell and Embryonal complications, Testicular Neoplasms pathology, Testicular Neoplasms physiopathology

Abstract

Male patients diagnosed with cancer are often referred for semen cryopreservation before gonadotoxic treatment but often have low semen quality. The aim of this study was to evaluate which type of cancer affects gonadal function and proposes a risk factor for low pre-treatment semen quality. Between January 1983 and August 2006, 764 male cancer patients were referred for semen cryopreservation prior to chemotherapy and radiotherapy. We compared semen characteristics and reproductive hormones between different groups of cancer patients. In addition, we evaluated the role of tumour markers in patients with testicular germ-cell tumours (TGCT) on fertility. Abnormal semen parameters were found in 489 men (64%) before cancer treatment. Patients with TGCT and extragonadal germ-cell tumours had significantly lower sperm concentrations and inhibin B levels than all other patient groups. No semen could be banked in 93 patients (12.2%). Eight hundred and thirty-nine of 927 (90%) produced semen samples were adequate for cryopreservation. Inhibin B in all groups showed to be the best predictor of semen quality. Although pre-treatment raised tumour markers were associated with a decrease in inhibin B and increased follicle stimulating hormone, both predictive for low semen quality; no direct linear association could be found between raised beta-HCG, alfa-fetoprotein and semen quality. Only 1/3 of cancer patients had normal semen parameters prior to cancer treatment. Patients with TGCT and extragonadal GCT have the highest risk for impaired semen quality and gonadal dysfunction at the time of semen cryopreservation.

Published

2010

8. Increased sperm DNA fragmentation in patients with vasectomy reversal has no prognostic value for pregnancy rate.

Author

Smit M, Wissenburg OG, Romijn JC, and Dohle GR

Subjects

Adult, Female, Humans, Male, Prognosis, Prospective Studies, DNA Fragmentation, Pregnancy statistics & numerical data, Spermatozoa, Vasovasostomy

Abstract

Purpose: We evaluated sperm DNA fragmentation in patients with vasectomy reversal and its prognostic value to determine spontaneous and assisted reproductive technique pregnancy rates., Materials and Methods: We prospectively assessed DNA fragmentation with the sperm chromatin structure assay in postoperative semen samples of 70 patients with vasectomy reversal. At a median +/- SD followup of 4.3 +/- 0.5 years pregnancy rates were recorded., Results: DNA fragmentation in patients with vasectomy reversal was significantly increased vs that in proven fertile controls (30.2% +/- 20.1% vs 15.3% +/- 5.4%, p <0.001). Significant negative correlations were found between DNA fragmentation index and total sperm count, progressive motility, total number of progressive sperm, normal morphology and sperm vitality (-0.325

Published

2010

9. Decreased sperm DNA fragmentation after surgical varicocelectomy is associated with increased pregnancy rate.

Author

Smit M, Romijn JC, Wildhagen MF, Veldhoven JL, Weber RF, and Dohle GR

Subjects

Adult, Female, Humans, Infertility, Male etiology, Male, Prospective Studies, Sperm Count, Sperm Motility, Urologic Surgical Procedures, Male methods, Varicocele complications, DNA Fragmentation, Infertility, Male genetics, Infertility, Male surgery, Pregnancy statistics & numerical data, Varicocele genetics, Varicocele surgery

Abstract

Purpose: We prospectively evaluated changes in sperm chromatin structure in infertile patients before and after surgical repair of varicocele, and the impact on the pregnancy rate., Materials and Methods: Included in the study were 49 men with at least a 1-year history of infertility, a palpable varicocele and oligospermia. World Health Organization semen analysis and sperm DNA damage expressed as the DNA fragmentation index using the sperm chromatin structure assay were assessed preoperatively and postoperatively. Pregnancy (spontaneous and after assisted reproductive technique) was recorded 2 years after surgery., Results: Mean sperm count, sperm concentration and sperm progressive motility improved significantly after varicocelectomy from 18.3 x 10(6) to 44.4 x 10(6), 4.8 x 10(6)/ml to 14.3 x 10(6)/ml and 16.7% to 26.6%, respectively (p <0.001). The DNA fragmentation index decreased significantly after surgery from 35.2% to 30.2% (p = 0.019). When the definition of greater than 50% improvement in sperm concentration after varicocelectomy was applied, 31 of 49 patients (63%) responded to varicocelectomy. After varicocelectomy 37% of the couples conceived spontaneously and 24% achieved pregnancy with assisted reproductive technique. The mean postoperative DNA fragmentation index was significantly higher in couples who did not conceive spontaneously or with assisted reproductive technique (p = 0.033)., Conclusions: After varicocelectomy sperm parameters significantly improved and sperm DNA fragmentation was significantly decreased. Low DNA fragmentation index values are associated with a higher pregnancy rate (spontaneous and with assisted reproductive technique). We suggest that varicocelectomy should be considered in infertile men with palpable varicocele, abnormal semen analysis and no major female factors.

Published

2010

10. Low folate in seminal plasma is associated with increased sperm DNA damage.

Author

Boxmeer JC, Smit M, Utomo E, Romijn JC, Eijkemans MJ, Lindemans J, Laven JS, Macklon NS, Steegers EA, and Steegers-Theunissen RP

Subjects

Adult, Humans, Male, Middle Aged, DNA Damage, Folic Acid analysis, Infertility, Male genetics, Infertility, Male metabolism, Semen chemistry, Spermatozoa metabolism

Abstract

Objective: To determine associations between vitamin B status, homocysteine (tHcy), semen parameters, and sperm DNA damage., Design: Observational study., Setting: A tertiary referral fertility clinic., Patient(s): Two hundred fifty-one men of couples undergoing in vitro fertilization (IVF) or intracytoplasmic sperm injection (ICSI) treatment, with subgroups of fertile (n = 70) and subfertile men (n = 63) defined according to semen concentration and proven fertility., Intervention(s): None., Main Outcome Measure(s): The DNA fragmentation index (DFI) as marker of sperm DNA damage determined using the sperm chromatin structure assay (SCSA), and semen parameters assessed according to World Health Organization criteria; tHcy, folate, cobalamin, and pyridoxine concentrations determined in seminal plasma and blood., Result(s): In the total group of fertile and subfertile men, all biomarkers in blood were statistically significantly correlated with those in seminal plasma. No correlation was found between the biomarkers in blood and the semen parameters. In seminal plasma, both tHcy and cobalamin positively correlated with sperm count. Folate, cobalamin, and pyridoxine were inversely correlated with ejaculate volume. In fertile men, seminal plasma folate showed an inverse correlation with the DNA fragmentation index., Conclusion(s): Low concentrations of folate in seminal plasma may be detrimental for sperm DNA stability.

Published

2009

11. Use rate and assisted reproduction technologies outcome of cryopreserved semen from 629 cancer patients.

Author

van Casteren NJ, van Santbrink EJ, van Inzen W, Romijn JC, and Dohle GR

Subjects

Adolescent, Adult, Female, Humans, Infertility, Male etiology, Live Birth, Male, Middle Aged, Pregnancy, Pregnancy Rate, Radiotherapy adverse effects, Retrospective Studies, Time Factors, Treatment Outcome, Young Adult, Antineoplastic Agents adverse effects, Cryopreservation statistics & numerical data, Infertility, Male therapy, Neoplasms therapy, Reproductive Techniques, Assisted statistics & numerical data, Semen Preservation statistics & numerical data, Sperm Banks statistics & numerical data

Abstract

Objective: To assess the use rate and assisted reproductive technologies (ART) outcome of the cryopreserved semen of cancer patients with an average follow-up of 7 years (range, 2-23 years)., Design: Retrospective data analysis., Setting: University-affiliated andrology and reproduction center., Patient(s): Six hundred twenty-nine male cancer patients who were referred for semen cryopreservation between 1983 and 2004., Intervention(s): Review of patient characteristics and ART outcome., Main Outcome Measure(s): Use rate and live births using cryopreserved semen., Result(s): A total of 749 semen samples from 557 men were preserved. Ninety-one patients died during follow-up, and another 29 requested disposal. Forty-two patients requested the use of their banked semen. ART data were available for 37 patients. A total of 101 ART cycles (32 IVF, 53 intracytoplasmic sperm injection [ICSIs], nine cryo-ET, and seven intrauterine inseminations [IUIs]) were performed, resulting in, respectively, 8, 16, 2, and 1 pregnancies. Pregnancies rates for IVF and ICSI were significantly higher than those for IUI., Conclusion(s): So far, 7.5% of the cancer survivors have used their banked semen, which led to live births in 49% of the couples. Semen cryopreservation is a reliable method to preserve fertility potential and gives couples a reasonable chance of achieving parenthood.

Published

2008

12. Semen cryopreservation in pubertal boys before gonadotoxic treatment and the role of endocrinologic evaluation in predicting sperm yield.

Author

van Casteren NJ, Dohle GR, Romijn JC, de Muinck Keizer-Schrama SM, Weber RF, and van den Heuvel-Eibrink MM

Subjects

Adolescent, Feasibility Studies, Humans, Male, Prognosis, Puberty, Time Factors, Cryopreservation methods, Gonadal Hormones blood, Infertility, Male rehabilitation, Semen Preservation methods, Sperm Count, Sperm Motility, Spermatozoa cytology

Abstract

Objective: To evaluate the feasibility of semen cryopreservation in pubertal boys before they receive gonadotoxic therapy and to identify which pretreatment parameters might predict successful cryopreservation., Design: Retrospective data analysis., Setting: Tertiary fertility center, academic children's hospital., Patient(s): Between 1995 and 2005, 80 boys (median age 16.6 years, range 13.7-18.9 years) consulted the outpatient clinic of andrology for semen cryopreservation before a potentially gonadotoxic treatment., Intervention(s): We assessed the pretreatment semen parameters, hormone levels, and patients' characteristics., Main Outcome Measure(s): Measurement of the number of adolescents able to cryopreserve semen., Result(s): Thirteen boys were unable to produce semen by masturbation. In 53 boys semen quality was adequate for cryopreservation. In 14 patients semen analysis did not show motile spermatozoa, and therefore semen cryopreservation could not be performed. Although inhibin B showed a strong correlation with sperm count, no significant difference was found in serum T, inhibin B, LH, and FSH levels in the patients with or without successful sperm yield. Moreover, median age was not different between patients with and without a successful sperm yield., Conclusion(s): Semen cryopreservation in boys is a feasible method to preserve spermatozoa before gonadotoxic therapy is started and should be offered to all pubertal boys despite their young age. Serum hormone levels do not predict sperm yield.

Published

2008

13. Seminal plasma cobalamin significantly correlates with sperm concentration in men undergoing IVF or ICSI procedures.

Author

Boxmeer JC, Smit M, Weber RF, Lindemans J, Romijn JC, Eijkemans MJ, Macklon NS, and Steegers-Theunissen RP

Subjects

Adult, Biomarkers analysis, Biomarkers blood, Folic Acid blood, Homocysteine blood, Humans, Infertility, Male etiology, Infertility, Male physiopathology, Male, Middle Aged, Pyridoxal Phosphate blood, Spermatogenesis physiology, Vitamin B 12 blood, Fertilization in Vitro, Semen chemistry, Sperm Count, Sperm Injections, Intracytoplasmic, Vitamin B 12 analysis

Abstract

Mild hyperhomocysteinemia is caused by B vitamin deficiencies. We hypothesize that these biochemical derangements detrimentally affect spermatogenesis. Therefore, the aim of this study was to investigate the folate, cobalamin, pyridoxine, and homocysteine concentrations in blood and seminal plasma and the associations between these biomarkers and semen parameters in men participating in an in vitro fertilization or intracytoplasmic sperm injection program. From 73 men (median age [range]: 37 years [28-53]), blood and semen samples were obtained for the determination of serum and red blood cell (RBC) folate, serum total cobalamin, whole-blood pyridoxal-5'-phosphate, plasma total homocysteine (tHcy), and serum total testosterone. Semen analysis included sperm concentration, motility, and morphology according to World Health Organization criteria. The B vitamins and tHcy concentrations were significantly correlated in blood but not in seminal plasma. The serum and RBC folate concentrations were significantly correlated also with the total folate concentration in seminal plasma (r = .44; P < .001 and r = .39; P < .001, respectively). Likewise, the total cobalamin concentration in serum and seminal plasma was significantly correlated (r = .55; P = .001). Of interest is that the total cobalamin concentration in seminal plasma was significantly correlated with the sperm concentration (r = .42; P < .001). This is in contrast to the absence of significant associations between the other vitamins and tHcy in blood and seminal plasma and any of the semen parameters. These findings suggest that folate and cobalamin are transferred from the blood to the male reproductive organs and emphasize the role of cobalamin in spermatogenesis in human.

Published

2007

14. Clinical correlates of the biological variation of sperm DNA fragmentation in infertile men attending an andrology outpatient clinic.

Author

Smit M, Dohle GR, Hop WC, Wildhagen MF, Weber RF, and Romijn JC

Subjects

Humans, Male, Outpatient Clinics, Hospital, Semen cytology, Sensitivity and Specificity, Sperm Count, Sperm Motility, Spermatozoa ultrastructure, Chromatin metabolism, DNA Fragmentation, Infertility, Male diagnosis, Spermatozoa metabolism

Abstract

Determination of sperm DNA fragmentation, as assessed by the sperm chromatin structure assay (SCSA), has become an important tool for the evaluation of semen quality. The aim of the present study was to describe the biological variation of sperm DNA fragmentation in men attending an andrology clinic and to identify clinical correlates of the biological variation of sperm DNA fragmentation. For this study, two consecutive semen samples from 100 patients attending our andrology outpatient clinic were subjected to semen analysis, performed in parallel according to WHO guidelines and by SCSA. A good agreement between pairs of samples was found for SCSA-derived variables, as indicated by a significantly lower median coefficient of variation (CV) of the DNA Fragmentation Index (DFI) and the high DNA stainability (HDS) compared with WHO semen parameters. In half of the men attending our andrology clinic, however, the individual biological variation of DFI and HDS, expressed as CV of two samples, exceeded 10%. Dysregulation of spermatogenesis, as seen as testicular insufficiency or varicocele, was not associated with increased variability of DFI or HDS. A backward multiple linear regression analysis, however, indicated that the biological variation of DFI may be more profound in men with characteristics of normal spermatogenesis. In conclusion, we confirm previous reports that sperm DNA fragmentation has a lower biological variability than classical semen parameters. We hypothesize that the sperm chromatin structure may be more influenced in patients with normal spermatogenesis, whereas in men with disturbed spermatogenesis, the chromatin structure may be already so impaired that the effect of unidentified factors leading to variability of sperm DNA fragmentation in time may not be as profound.

Published

2007

15. Androgen receptor modifications in prostate cancer cells upon long-termandrogen ablation and antiandrogen treatment.

Author

Marques RB, Erkens-Schulze S, de Ridder CM, Hermans KG, Waltering K, Visakorpi T, Trapman J, Romijn JC, van Weerden WM, and Jenster G

Subjects

Androgen Antagonists therapeutic use, Androgens pharmacology, Animals, Cell Division drug effects, Cell Line, Tumor, Down-Regulation, Flutamide therapeutic use, Gene Expression Regulation, Neoplastic, Humans, Male, Mice, Mice, Nude, Mutation, Orchiectomy, Prostatic Neoplasms drug therapy, Prostatic Neoplasms genetics, Transplantation, Heterologous, Prostatic Neoplasms pathology, Receptors, Androgen genetics

Abstract

To study the mechanisms whereby androgen-dependent tumors relapse in patients undergoing androgen blockade, we developed a novel progression model for prostate cancer. The PC346C cell line, established from a transurethral resection of a primary tumor, expresses wild-type (wt) androgen receptor (AR) and secretes prostate-specific antigen (PSA). Optimal proliferation of PC346C requires androgens and is inhibited by the antiandrogen hydroxyflutamide. Orthotopic injection in the dorsal-lateral prostate of castrated athymic nude mice did not produce tumors, whereas fast tumor growth occurred in sham-operated males. Three androgen-independent sublines were derived from PC346C upon long-term in vitro androgen deprivation: PC346DCC, PC346Flu1 and PC346Flu2. PC346DCC exhibited androgen-insensitive growth, which was not inhibited by flutamide. AR and PSA were detected at very low levels, coinciding with background AR activity in a reporter assay, which suggests that these cells have bypassed the AR pathway. PC346Flu1 and PC346Flu2 were derived by culture in steroid-stripped medium supplemented with hydroxyflutamide. PC346Flu1 strongly upregulated AR expression and showed 10-fold higher AR activation than the parental PC346C. PC346Flu1 proliferation was inhibited in vitro by R1881 at 0.1 nM concentration, consistent with a slower tumor growth rate in intact males than in castrated mice. PC346Flu2 carries the well-known T877A AR mutation, causing the receptor to become activated by diverse nonandrogenic ligands including hydroxyflutamide. Array-based comparative genomic hybridization revealed little change between the various PC346 lines. The common alterations include gain of chromosomes 1, 7 and 8q and loss of 13q, which are frequently found in prostate cancer. In conclusion, by in vitro hormone manipulations of a unique androgen-dependent cell line expressing wtAR, we successfully reproduced common AR modifications observed in hormone-refractory prostate cancer: downregulation, overexpression and mutation.

Published

2005

16. Clinical laboratory evaluation of male subfertility.

Author

Weber RF, Dohle GR, and Romijn JC

Subjects

Fertilization, Gonadotropins, Pituitary analysis, Humans, Male, Spermatozoa cytology, Spermatozoa physiology, Infertility, Male diagnosis

Abstract

Male subfertility is a common problem with a complex etiology, requiring a complete andrological work-up for proper diagnosis. The male reproductive tract is controlled by a well-balanced hormonal system, in which hypothalamic (GnRH), pituitary (LH, FSH) and testicular hormones (androgens, inhibin B) participate. Any disturbance of this hormonal system may therefore lead to testicular dysfunction and interfere with the spermatogenesis process. In addition, also other components along the ductal system, such as epididymis, prostate and seminal vesicles, that improve sperm fertility by contributing their secretions to the semen, might function inadequately and thus fail to enhance the fertilizing capacity of the sperm cells. External factors (heat, chemicals, life style) and anatomical abnormalities (varicocele) were shown to have a negative influence on male fertility. In a number of patients genetic defects can be identified as the cause of their infertility. Laboratory tests are available to assess hormone concentrations, semen composition, accessory gland function and sperm cell function. Conventional semen analysis includes the determination of sperm concentration, semen volume, sperm motility (qualitative and quantitative), sperm morphology, sperm cell vitality, pH, leucocytes and antibodies. The usefulness of the determination of these parameters as predictor of fertility appears to be rather limited, however. Therefore, alternative tests, some based on more functional aspects (sperm penetration, capacitation, acrosome reaction), have been developed. Furthermore, there is an increasing attention for the assessment of DNA integrity, for instance by the flowcytometer-based Sperm Chromation Structure Assay (SCSA), as an additional or alternative parameter of sperm quality. It is likely and desirable that further assays with better predictive value are being developed in the near future.

Published

2005

17. Internalization of calcium oxalate crystals by renal tubular cells: a nephron segment-specific process?

Author

Schepers MS, Duim RA, Asselman M, Romijn JC, Schröder FH, and Verkoelen CF

Subjects

Animals, Calcium Oxalate chemistry, Carbon Radioisotopes, Cell Line, Crystallization, Epithelial Cells metabolism, Epithelial Cells ultrastructure, Fixatives, Hyaluronic Acid metabolism, Hyaluronoglucosaminidase, Kidney Tubules cytology, Microscopy, Confocal, Microscopy, Electron, Microscopy, Phase-Contrast, Nephrons cytology, Calcium Oxalate pharmacokinetics, Kidney Tubules metabolism, Nephrons metabolism

Abstract

Background: Crystal retention in the kidney is caused by the interaction between crystals and the cells lining the renal tubules. These interactions involve crystal attachment, followed by internalization or not. Here, we studied the ability of various renal tubular cell lines to internalize calcium oxalate monohydrate (COM) crystals., Methods: Crystal-cell interactions are studied by light-, electron-, and confocal microscopy with cells resembling the renal proximal tubule [porcine kidney (LLC-PK1)], proximal/distal tubule [Madin-Darby canine kidney II (MDCK-II)], and distal tubule and/or collecting ducts [(Madin-Darby canine kidney I (MDCK-I), rat cortical collecting duct 1 (RCCD1)]. Crystal-binding strength and internalization are characterized and quantified with radiolabeled COM., Results: Microscopy studies showed that crystals were firmly embedded in the membranes of LLC-PK1 and MDCK-II cells to be subsequently internalized. On the other hand, crystals bound only loosely to MDCK-I and RCCD1 and were not taken up by these cells. Crystal uptake by LLC-PK1 and MDCK-II, expressed in microg/10(6) cells, is temperature-dependent and gradually increases from 0.88 and 0.15 in 30 minutes, respectively, to 4.70 and 3.85, respectively, after five hours, whereas these values never exceeded background levels in MDCK-I and RCCD1 cells., Conclusion: The adherence of COM crystals to renal cells with properties of the proximal tubule is inevitable and actively followed by their uptake, whereas crystals attached to cells resembling the distal tubule and/or collecting duct are not internalized. Since crystal formation usually occurs in segments beyond the renal proximal tubule, crystal uptake may be of less importance in the etiology of idiopathic calcium oxalate stone disease.

Published

2003

18. Polyamines and prostatic cancer.

Author

Schipper RG, Romijn JC, Cuijpers VM, and Verhofstad AA

Subjects

Antineoplastic Agents pharmacology, Biogenic Polyamines antagonists & inhibitors, Biomarkers, Tumor, Cell Division drug effects, Homeostasis drug effects, Humans, Male, Prostatic Neoplasms drug therapy, Biogenic Polyamines physiology, Prostatic Neoplasms pathology

Abstract

The importance of polyamines in prostatic growth and differentiation has prompted studies to evaluate the clinical relevance of the ornithine decarboxylase/polyamine system in prostatic cancer. These studies show that differences in biological behaviour of prostatic (cancer) cells are associated with changes in polyamine levels and/or the activity of their metabolic enzymes. Faulty antizyme regulation of polyamine homoeostasis may play an important role in the growth and progression of prostatic carcinoma. Treatment of human prostate carcinoma cells with inhibitors of polyamine metabolic enzymes or polyamine analogues induces cell growth arrest or (apoptotic) cell death. Our recent in vitro studies using conformationally restricted polyamine analogues show that these compounds inhibit cell growth, probably by inducing antizyme-mediated degradation of ornithine decarboxylase. Sensitivity of human prostate cancer cells for these compounds was increased in the absence of androgens. These results suggest that these analogues might have chemotherapeutic potential in case prostatic cancer has become androgen-independent. Pilot data in an in vivo model show that these analogues have effects on tumour cell proliferation, vascularity, blood perfusion and tissue hypoxia. Overall, these studies show that polyamines may serve as important biomarkers of prostatic malignancy and provide a promising target for chemotherapy of prostatic cancer.

Published

2003

19. Pericellular matrix formation by renal tubule epithelial cells in relation to crystal binding.

Author

Schepers MS, Asselman M, Duim RA, Romijn JC, Schröder FH, and Verkoelen CF

Subjects

Animals, Calcium Oxalate chemistry, Cell Line, Crystallization, Dogs, Epithelial Cells cytology, Epithelial Cells metabolism, Hyaluronan Receptors metabolism, Hyaluronic Acid biosynthesis, Kidney Tubules cytology, Calcium Oxalate metabolism, Extracellular Matrix metabolism, Hyaluronic Acid metabolism, Kidney Tubules metabolism

Abstract

Background/aim: Retention of crystals in the kidney ultimately leads to renal stone formation. Hyaluronan (HA) has been identified as binding molecule for calcium oxalate monohydrate crystals. The association of high molecular mass (M(r)) HA with cell surface receptors such as CD44 gives rise to pericellular matrix (PCM) formation by many eukaryotic cells in culture. Here, we study the ability of several renal tubular cell lines to assemble PCMs and to synthesize high-M(r) HA during proliferation in relation to crystal retention., Methods: PCM assembly by MDCK-I, MDCK-II, and LLC-PK1 cells was visualized by particle exclusion assay. Metabolic labeling studies were performed to estimate the cellular production of HA. The expression of CD44 and HA was studied using fluorescent probes, and crystal binding was quantified with radiolabeled calcium oxalate monohydrate., Results: PCMs were formed, and HA was expressed by most MDCK-I and some MDCK-II, but not by LLC-PK1 cells. All cell types expressed CD44 at their apical surface. MDCK-I and MDCK-II cells secreted, respectively, 14.7 +/- 1.6 and 0.5 +/- 0.2 pmol [3H]glucosamine incorporated in high-M(r) HA, whereas LLC-PK1 cells did not secrete HA. Streptomyces hyaluronidase treatment significantly decreased crystal binding (microg/cm2) to MDCK-I cells (from 8.6 +/- 0.4 to 3.9 +/- 0.9), but hardly to MDCK-II cells (from 10.2 +/- 0.2 to 9.6 +/- 0.1) or LLC-PK1 cells (from 10.2 +/- 0.8 to 9.9 +/- 0.3)., Conclusions: There are various forms of crystal binding to renal tubular cells in culture. Crystal attachment to MDCK-I and some MDCK-II cells involves PCM assembly that requires high-M(r) HA synthesis. HA production and PCM formation do not play a role in crystal binding to LLC-PK1 and the majority of MDCK-II cells. It remains to be determined which form of binding is involved in renal stone disease., (Copyright 2003 S. Karger AG, Basel)

Published

2003

20. Urinary crystallization inhibitors do not prevent crystal binding.

Author

Schepers MS, van der Boom BG, Romijn JC, Schröder FH, and Verkoelen CF

Subjects

Animals, Cells, Cultured, Crystallization, Dogs, Humans, Swine, Urine, Calcium Oxalate pharmacology, Hyaluronic Acid pharmacology, Kidney cytology, Kidney drug effects, Kidney Calculi etiology, LLC-PK1 Cells drug effects

Abstract

Purpose: Renal stone formation requires the persistent retention of crystals in the kidney. Calcium oxalate monohydrate (COM) crystal binding to Madin Darby canine kidney strain I (MDCK-I), a cell line that resembles the epithelium in the renal distal tubule/collecting duct, is developmentally regulated, while LLC-PK1 cells (American Type Tissue Collection), which are widely used as a model of the renal proximal tubule, bind crystals irrespective of their stage of epithelial development. Whereas to our knowledge the binding molecules for COM at the surface of LLC-PK1 cells are still unknown, crystals adhere to the hyaluronan (HA) rich pericellular matrix transiently expressed by mobile MDCK-I cells. In the current study we investigated whether crystal binding to either cell type is influenced by urinary substances, including glycoprotein inhibitors of crystallization, Materials and Methods: We studied crystal binding to MDCK-I cells during wound repair, to confluent LLC-PK1 cells and to HA immobilized on a solid surface using [14C] COM pretreated or not pretreated with urine from healthy male volunteers. Sodium dodecyl sulfate-polyacrylamide gel electrophoresis and Western blot analysis were performed to assess whether the crystals became coated with urine derived proteins, Results: Western blot analysis demonstrated that pretreated COM crystals were covered with protein inhibitors of crystallization. However, this protein coat had no significant effect on the level of crystal binding to either cell type. In contrast, the adherence of urine treated crystals to immobilized HA was significantly reduced, Conclusions: The adherence of crystals to pericellular matrixes may encompass more than their simple fixation to the polysaccharide HA. Calcium oxalate crystal retention is not prevented by coating crystals with urinary constituents such as glycoproteins and, therefore, may predominantly depend on the surface properties of the renal tubular epithelium.

Published

2002

21. Inhibition of apoptotic proteins causes multidrug resistance in renal carcinoma cells.

Author

Scheltema JM, Romijn JC, van Steenbrugge GJ, Schröder FH, and Mickisch GH

Subjects

Amsacrine pharmacology, Antineoplastic Agents pharmacology, Apoptosis physiology, Carcinoma, Renal Cell metabolism, Carcinoma, Renal Cell pathology, Enzyme Inhibitors pharmacology, Etoposide pharmacology, Humans, Kidney Neoplasms metabolism, Kidney Neoplasms pathology, Proto-Oncogene Proteins antagonists & inhibitors, Proto-Oncogene Proteins biosynthesis, Proto-Oncogene Proteins c-bcl-2 antagonists & inhibitors, Proto-Oncogene Proteins c-bcl-2 biosynthesis, Topoisomerase II Inhibitors, Tumor Cells, Cultured, bcl-2-Associated X Protein, Apoptosis drug effects, Carcinoma, Renal Cell drug therapy, Drug Resistance, Multiple, Kidney Neoplasms drug therapy

Abstract

Renal Cell Carcinomas (RCCs) exhibit strong resistance to the most chemotherapeutic treatments probably due to the expression of various multidrug resistance (MDR) genes. Overexpression of P-glycoprotein (Pgp) is established as one such factor, but other mechanisms such as at-MDR, characterized by attenuated DNA-topoisomerase II (topoII) activity, may be functional as well. In addition, regulating proteins involved in apoptosis can exhibit multidrug resistant features. However, prevention of apoptosis as a mechanism of MDR has not yet been assessed in RCC, nor has the cytotoxicity of a variety of chemotherapeutic agents known to trigger apoptotic or necrotic cell death been tested in RCC in a systematic fashion. Using immunohistochemistry and Western blotting, Bcl-2 and Bax expression was determined in a panel of multidrug resistant RCC lines featuring Pgp and/or at-MDR. The results were related to apoptotic activity and kind of cell death in these cell lines, demonstrated by incubation with Hoechst 33342 and propidium iodide after treatment with various cytotoxic agents and quantitated by MTT. In the drug resistant sublines, some decreased Bax and strongly increased Bcl-2 expression was seen by immunohistochemistry indicating prevention of apoptosis as a distinct feature of MDR in RCC. This was confirmed by Western blotting. Sublines revealed significant resistance for all drugs, except for CC-313 and DiMIQ. However, these drugs induced necrotic cell death, in contrast to all other drugs tested, which induced apoptotic cell death. We conclude that, in chemoselected RCC sublines, multidrug resistance appears to be functional due to inhibition of apoptosis, apart from the MDR1 and at-MDR resistance mechanisms. CC-313 and DiMIQ are very potent cytotoxic agents in RCC, probably because they do not kill by induction of apoptosis.

Published

2001

22. Identification of hyaluronan as a crystal-binding molecule at the surface of migrating and proliferating MDCK cells.

Author

Verkoelen CF, Van Der Boom BG, and Romijn JC

Subjects

Animals, Carbon Radioisotopes, Cell Division physiology, Cell Line, Chondroitinases and Chondroitin Lyases pharmacology, Crystallization, Dogs, Epithelial Cells chemistry, Epithelial Cells cytology, Epithelial Cells metabolism, Glycosaminoglycans metabolism, Hyaluronic Acid analysis, Hyaluronic Acid chemistry, Hyaluronoglucosaminidase pharmacology, Kidney Calculi chemistry, Kidney Calculi metabolism, Plastics, Protein Binding drug effects, Protein Binding physiology, Wound Healing physiology, Calcium Oxalate chemistry, Calcium Oxalate metabolism, Cell Movement physiology, Hyaluronic Acid metabolism, Kidney cytology

Abstract

Background: The adherence of calcium oxalate crystals to the renal tubule epithelium is considered a critical event in the pathophysiology of calcium nephrolithiasis. Calcium oxalate monohydrate (COM) crystals cannot adhere to the surface of a functional Madin-Darby canine kidney (MDCK) monolayer, but they bind avidly to the surface of proliferating and migrating cells., Methods: To identify crystal-binding molecules (CBMs) at the surface of crystal-attracting cells, we applied metabolic labeling protocols in combination with differential enzymatic digestion and gel filtration, which was compared with [14C]COM crystal binding and confirmed by confocal microscopy., Results: The indication that hyaluronan [hyaluronic acid (HA)] might act as a CBM in subconfluent cultures came from studies with glycosaminoglycan (GAG)-degrading enzymes. Subsequently, metabolic-labeling studies revealed that hyaluronidase cleaved significantly more radiolabeled glycoconjugates from crystal-attracting cells than from cells without affinity for crystals. During wound repair, crystal binding could be prevented by pretreating the healing cultures with hyaluronate lyase, an enzyme that specifically hydrolyzes HA. Binding to immobilized HA provided evidence that COM crystals physically can become associated with this polysaccharide. Finally, confocal microscopy demonstrated that fluorescently labeled HA binding protein (HABP) adhered to the surface of proliferating cells in subconfluent cultures as well as to cells involved in closing a wound, but not to cells in confluent monolayers., Conclusions: These results identify HA as binding molecule for COM crystals at the surface of migrating and proliferating MDCK cells.

Published

2000

23. Use of nude mouse xenograft models in prostate cancer research.

Author

van Weerden WM and Romijn JC

Subjects

Animals, Humans, Male, Mice, Mice, Nude, Transplantation, Heterologous, Tumor Cells, Cultured, Models, Biological, Prostatic Neoplasms physiopathology

Abstract

Background: Our understanding of the mechanisms of (progressive) growth of prostatic cancer has been largely obtained through the study of experimental animal models. To be able to validate new concepts, representative model systems of human origin that mimic the clinical process of the disease in patients are essential. Unfortunately, the limited number of human prostate tumor models has considerably hampered research., Methods: Various research groups have put much effort in the development of human prostate tumor xenograft models, and large numbers of clinical prostate tumors were heterotransplanted in immune-deficient host animals. This huge effort has resulted in a number of tumor lines which are reviewed here., Results: Up to now, approximately 25 xenograft models of human prostate cancer have been established and reported in the literature. The available xenografts seem to represent the various stages of clinical prostate cancer, such as early progression and transition from androgen-dependent to androgen-independent growth. In addition, recent efforts are concentrating on the establishment of in vitro cell lines from these xenografts as well as on the development of (bone) metastatic variants., Conclusions: Xenograft models are important for elucidating regulatory pathways of tumor growth and progression and are indispensible for testing of new treatment modalities., (Copyright 2000 Wiley-Liss, Inc.)

Published

2000

24. Sialic acid and crystal binding.

Author

Verkoelen CF, van der Boom BG, Kok DJ, and Romijn JC

Subjects

Animals, Binding, Competitive, Cell Line, Crystallization, Dogs, Kidney cytology, Lactose analogs & derivatives, Lactose pharmacology, Lectins metabolism, N-Acetylneuraminic Acid pharmacology, Neuraminidase pharmacology, Sialic Acids pharmacology, Calcium Oxalate metabolism, Kidney metabolism, N-Acetylneuraminic Acid physiology

Abstract

Background: We studied the role of cell surface sialic acid in the adherence of calcium oxalate monohydrate (COM) crystals to Madin-Darby canine kidney (MDCK) cells., Methods: Studies were performed with undifferentiated (crystal-binding) cells in subconfluent cultures and maturated (noncrystal-binding) cells in confluent cultures. Lectins were used to study the emergence and abundance of oligosaccharides at the cell surface during epithelial development. The effect of neuraminidase treatment on crystal binding was studied with [14C]COM crystals, and the enzyme-induced release of cell surface-associated sialic acid molecules was monitored by labeling the cells metabolically with [3H]glucosamine., Results: Binding studies with lectins derived from Maackia Amurensis II (MALII) and Sambucus Nigra (SNA) demonstrated that the cells expressed terminal sialic acids attached to penultimate galactose through alpha 2,3 and alpha 2,6 bonds at different stages of epithelial development. Neuraminidase treatment strongly reduced the affinity of the cell surface for COM crystals in subconfluent cultures. Nevertheless, neuraminidase cleaved more sialic acids from cells in confluent cultures than from those in subconfluent cultures. Peanut agglutinin (PNA), which binds only to sialylated terminal galactose units, adhered to developing but not to maturated cells, unless the latter were pretreated with neuraminidase. Both results indicate that the surface of maturated MDCK cells is more heavily sialylated than that of undifferentiated cells. Free sialic acid molecules showed little or no affinity for COM crystals and did not affect the adherence of the crystals to undifferentiated cells., Conclusions: There are at least two models that may explain these results. First, sialic acids are presented at the surface of immature cells in an orientation that specifically matches crystal surface characteristics favoring crystal-cell interactions. Second, sialic acid molecules are not directly associated with the crystals, but may be involved in the exposure of another crystal binding molecule at the cell surface.

Published

2000

25. Androgen-independent growth is induced by neuropeptides in human prostate cancer cell lines.

Author

Jongsma J, Oomen MH, Noordzij MA, Romijn JC, van Der Kwast TH, Schröder FH, and van Steenbrugge GJ

Subjects

Cell Division drug effects, Cyclic AMP physiology, Dideoxyadenosine pharmacology, Enzyme Inhibitors pharmacology, Gastrin-Releasing Peptide pharmacology, Humans, Male, Oxadiazoles pharmacology, Proto-Oncogene Proteins c-bcl-2 metabolism, Quinoxalines pharmacology, Thymidine metabolism, Tumor Cells, Cultured drug effects, Tumor Cells, Cultured pathology, Androgens physiology, Neuropeptides physiology, Prostatic Neoplasms metabolism, Prostatic Neoplasms pathology

Abstract

Background: Androgen-independent growth leads to progressive prostate cancer after androgen-ablation therapy. This may be caused by altered specificity of the androgen receptor (AR), by ligand-independent stimulation of the AR, or by paracrine growth modulation by neuropeptides secreted by neuroendocrine (NE) cells., Methods: We established and characterized the androgen-independent FGC-DCC from the androgen-dependent LNCaP fast growing colony (FGC) cell line. The androgen-independent DU-145, FGC-DCC, and PC-3, and the androgen-dependent LNCaP and PC-346C cell lines were used to study growth modulation of gastrin-releasing peptide (GRP), calcitonin (CT), serotonin (5-HT), and vasoactive intestinal peptide (VIP) by (3)H-thymidine incorporation. Specificity of the growth-modulating effects was tested with the anti-GRP monoclonal antibody 2A11 and induction of cAMP by neuropeptides., Results: Androgen-independent growth stimulation by neuropeptides was shown in DU-145 and PC-346C. 2A11 inhibited GRP-induced (3)H-thymidine incorporation in DU-145 and PC-346C and inhibited proliferation of the FGC-DCC and PC-3 cell lines. With some exceptions, cAMP induction paralleled growth stimulation. Dideoxyadenosine (DDA) inhibited the GRP-induced growth effect in DU-145 and PC-346C, whereas oxadiazoloquinoxaline-1-one (ODQ) had no effect on (3)H-thymidine incorporation. None of the neuropeptides stimulated growth of LNCaP, FGC-DCC, or PC-3., Conclusions: GRP-induced growth of DU-145 and PC-346C was specific and cAMP-mediated. Androgen-independent growth of FGC-DCC cells was mainly due to an induction of Bcl-2 expression and possibly through the activation of an autocrine and NE-like pathway, as has been shown also for the PC-3 cell line. Growth induction of non-NE cells by neuropeptides could be a possible role for NE cells in clinical prostate cancer., (Copyright 2000 Wiley-Liss, Inc.)

Published

2000

26. An Sp1 binding site is essential for basal activity of the human prostate-specific transglutaminase gene (TGM4) promoter.

Author

Dubbink HJ, Cleutjens KB, van der Korput HA, Trapman J, and Romijn JC

Subjects

Base Sequence, Binding Sites genetics, Binding, Competitive, DNA genetics, DNA metabolism, DNA-Binding Proteins metabolism, Electrophoresis, Polyacrylamide Gel, Humans, Luciferases genetics, Luciferases metabolism, Male, Molecular Sequence Data, Mutation, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Sequence Deletion, Sp3 Transcription Factor, Transcription Factors metabolism, Transglutaminases chemistry, Transglutaminases metabolism, Tumor Cells, Cultured, Promoter Regions, Genetic genetics, Prostate enzymology, Sp1 Transcription Factor metabolism, Transglutaminases genetics

Abstract

Human prostate-specific transglutaminase (hTG(P)) is a cross-linking enzyme encoded by the TGM4 gene. The TGM4 gene promoter was characterized by deletion mapping and mutational analysis. Promoter constructs, containing the minimal promoter requirements, could efficiently drive transcription in the prostate cancer cell lines PC346C and LNCaP and the hepatic cancer cell line Hep3B. The region between positions -113 and -61 was demonstrated to be essential for core promoter activity. Further analysis revealed the functional importance of an Sp1 binding motif, 5'-ACCCCGCCCC-3', at positions -96 to -87. This sequence is a binding site of the ubiquitous transcription factors Sp1 and Sp3.

Published

1999

27. Attachment sites for particles in the urinary tract.

Author

Verkoelen CF, Van Der Boom BG, Kok DJ, Schroder FH, and Romijn JC

Subjects

Animals, Annexin A5 metabolism, Binding Sites, Cells, Cultured, Crystallization, Dogs, N-Acetylneuraminic Acid physiology, Phosphatidylserines physiology, Calcium Oxalate chemistry, Kidney metabolism, Kidney Calculi etiology

Abstract

The adherence of crystals to the surface of renal tubule epithelial cells is one of the initial events in the development of nephrolithiasis. The accumulation of crystalline material in the kidney will sooner or later result in the formation of a stone. Calcium crystals occasionally are present in the urine of even healthy individuals, and mechanisms responsible for the selective attachment of crystals to the tubular epithelium of stone-forming individuals must exist. Although several types of cell surface molecules, including phosphatidylserine (PS) and sialic acid, have been proposed as receptors for crystals in the tubular system, the exact nature of these crystal-binding sites has not yet been revealed. Previously, it was demonstrated that calcium oxalate monohydrate crystals adhere to subconfluent, but not to confluent, Madin-Darby canine kidney-I cultures. This model was used here to investigate whether the surface of cells with affinity for crystals is enriched with one of the proposed crystal-binding molecules. Annexin V was used for the detection of PS at the cell surface, and Sambucus nigra lectin was used to reveal terminal sialic acid in a (alpha2,6) linkage to galactose units. FITC-annexin V binding studies showed that PS was not exposed at the surface of proliferating or growth-inhibited cells, unless they were pretreated with an apoptosis-inducing cytotoxic agent. Sambucus nigra lectin binding, of which the specificity was confirmed by blocking with N-acetylneuraminyl-lactose, demonstrated the abundant presence of (alpha2,6)-linked sialic acid residues at the cell surface of both subconfluent and confluent cultures. While these results seem to rule out a role for PS in the adherence of calcium oxalate monohydrate crystals to the surface of maturating Madin-Darby canine kidney-I cells, they question the role for cell surface-associated sialylated glycoconjugates in this process.

Published

1999

28. LLC-PK1 cells as a model system to study proximal tubule transport of water and other compounds relevant for renal stone disease.

Author

Verkoelen CF, Kok DJ, van der Boom BG, de Jonge HR, Schröder FH, and Romijn JC

Subjects

Animals, Biological Transport, Electrolytes metabolism, Inulin metabolism, Osmolar Concentration, Oxalates metabolism, Swine, Time Factors, Kidney Calculi metabolism, Kidney Tubules, Proximal metabolism, LLC-PK1 Cells, Water metabolism

Abstract

LLC-PK1 cells were cultured on a permeable support in a two-compartment culture system. Confluent monolayers received an ultrafiltrate-like solution at the apical side and a plasma-like solution at the basolateral side. The distribution of various solutes, including phosphate, calcium, and oxalate over both compartments was measured in time. The transport of water was monitored by alterations in fluid concentrations of radiolabeled inulin. Bicarbonate, glucose, and phosphate were transported rapidly from the apical to basolateral side of the monolayer. Sodium and chloride were reabsorbed without major consequences for the osmolality in the apical and basal fluid. Calcium and potassium were also reabsorbed, but to a smaller extent than sodium. The luminal concentration of oxalate gradually increased to values that were at least three times higher (12.0+/-0.4 micromol/l) than those in the contraluminal fluid (3.8+/-0.1 micromol/l). However, since the luminal rise of oxalate completely matched the rise of inulin in the apical fluid this appeared to be the passive consequence of active water reabsorption rather than of net directed oxalate transport. The LLC-PK1 model could prove useful to study the regulation of proximal tubule water transport and its effect on luminal stone salt concentrations under different physiological conditions.

Published

1999

29. Cell type-specific acquired protection from crystal adherence by renal tubule cells in culture.

Author

Verkoelen CF, van der Boom BG, Kok DJ, Houtsmuller AB, Visser P, Schröder FH, and Romijn JC

Subjects

Animals, Calcium Oxalate metabolism, Cell Adhesion physiology, Cell Line, Cell Size physiology, Crystallization, Diffusion Chambers, Culture, Dogs, Kidney Tubules, Collecting cytology, Kidney Tubules, Collecting ultrastructure, Kidney Tubules, Proximal cytology, Kidney Tubules, Proximal ultrastructure, LLC-PK1 Cells, Microscopy, Confocal, Microscopy, Electron, Scanning, Ouabain metabolism, Sodium-Potassium-Exchanging ATPase metabolism, Swine, Time Factors, Kidney Tubules, Collecting metabolism, Kidney Tubules, Proximal metabolism

Abstract

Background: Adherence of crystals to the surface of renal tubule epithelial cells is considered an important step in the development of nephrolithiasis. Previously, we demonstrated that functional monolayers formed by the renal tubule cell line, Madin-Darby canine kidney (MDCK), acquire protection against the adherence of calcium oxalate monohydrate crystals. We now examined whether this property is cell type specific. The susceptibility of the cells to crystal binding was further studied under different culture conditions., Methods: Cell-type specificity and the influence of the growth substrate was tested by comparing calcium oxalate monohydrate crystal binding to LLC-PK1 cells and to two MDCK strains cultured on either permeable or impermeable supports. These cell lines are representative for the renal proximal tubule (LLC-PK1) and distal tubule/collecting duct (MDCK) segments of the nephron, in which crystals are expected to be absent and present, respectively., Results: Whereas relatively large amounts of crystals adhered to subconfluent MDCK cultures, the level of crystal binding to confluent monolayers was reduced for both MDCK strains. On permeable supports, MDCK cells not only obtained a higher level of morphological differentiation, but also acquired a higher degree of protection than on impermeable surfaces. Crystals avidly adhered to LLC-PK1 cells, irrespective of their developmental stage or growth substrate used., Conclusions: These results show that the prevention of crystal binding is cell type specific and expressed only by differentiated MDCK cells. The anti-adherence properties acquired by MDCK cells may mirror a specific functional characteristic of its in situ equivalent, the renal distal tubule/collecting ducts.

Published

1999

30. Chemosensitivity of prostate cancer cell lines and expression of multidrug resistance-related proteins.

Author

van Brussel JP, van Steenbrugge GJ, Romijn JC, Schröder FH, and Mickisch GH

Subjects

ATP Binding Cassette Transporter, Subfamily B, Member 1 metabolism, Blotting, Western, DNA Topoisomerases, Type I metabolism, Drug Resistance, Multiple, Drug Resistance, Neoplasm, Glutathione Transferase metabolism, Humans, Immunohistochemistry, Male, Proto-Oncogene Proteins metabolism, Proto-Oncogene Proteins c-bcl-2 metabolism, Tumor Cells, Cultured, bcl-2-Associated X Protein, Neoplasm Proteins metabolism, Prostatic Neoplasms drug therapy, Prostatic Neoplasms metabolism

Abstract

The aim of this study was to obtain insight into the role of the multidrug resistance (MDR) phenomenon in hormone-independent progressive prostate cancer. Using immunocytochemistry and Western blotting we determined the expression of P-glycoprotein (Pgp), multidrug resistance-associated protein (MRP), glutathione-S-transferase-pi (GST-pi), Bcl-2, Bax, topoisomerase (Topo) I, II alpha and II beta in the human prostate cancer cell lines PC3, TSU-Pr1, DU145 and LNCaP derivatives LNCaP-R, LNCaP-LNO and LNCaP-FGC. Proliferative activity was assessed by immunocytochemistry. MTT assays were used to determine the sensitivity to etoposide, doxorubicin and vinblastin. Pgp was not expressed in any of the cell lines. MRP was variably expressed. GST-pi was expressed in TSU-Pr1, PC3 and DU145. The expression of Bcl-2 was restricted to TSU-Pr1, whereas Bax was found in all cell lines. Topo II alpha was expressed at the highest level in the rapidly proliferating cell lines TSU-Pr1 and DU145. Topo I and II beta were equally expressed. Resistance profiles varied among the cell lines, with TSU-Pr1 being the most sensitive and LNCaP-LNO relatively resistant. Multiple MDR proteins were expressed in prostate cancer cell lines and may well influence response to chemotherapy. Future functional studies, using chemo-selected MDR models, may further help to determine the mechanism or combination of mechanisms underlying the resistance of prostate cancer to chemotherapy.

Published

1999

31. Human prostate-specific transglutaminase: a new prostatic marker with a unique distribution pattern.

Author

Dubbink HJ, Hoedemaeker RF, van der Kwast TH, Schröder FH, and Romijn JC

Subjects

Biomarkers, Biopsy, Needle, Blotting, Western, Body Fluids enzymology, Humans, Immunohistochemistry, Male, Prostate pathology, Reference Values, Semen enzymology, Seminal Vesicles enzymology, Tissue Distribution, Androgen-Binding Protein metabolism, Prostate enzymology

Abstract

Human prostate-specific transglutaminase (hTGp) is a cross-linking enzyme, the physiologic function of which has not been established unequivocally yet. To gain insight into its distribution, we raised antisera against hTGp. By using Western blotting analysis, we found that these antisera specifically recognize a 77-kDa protein in prostatic fluids, seminal plasmas, and prostatic tissues. The concentrations of hTGp in these fluids and tissues were found to be highly variable among individuals. Immunohistochemical examination of several formalin-fixed paraffin-embedded human tissues revealed an exclusive expression in the prostate. The histologic localization and distribution of hTGp within the prostate was assessed by studying multiple sections from tumor-containing prostatectomy specimens and needle biopsies. hTGp expression was entirely restricted to luminal epithelial cells. No basal epithelial cells or stromal cells were stained. Within the prostate, large areas without any hTGp-positive cells were seen. Immunopositive cells were present either in a scattered pattern or concentrated in single or multiple glands in which all luminal epithelial cells expressed hTGp. The latter staining pattern occurred frequently, but not exclusively, in the peripheral zone, whereas scattered expression was most often observed in the transitional zone. Expression of the hTGp protein could occasionally be observed in high-grade prostatic intraepithelial neoplasia, but was not detected in prostate carcinoma cells. The expression pattern as observed for hTGp has not been found thus far for any other prostate-specific marker.

Published

1999

32. Down-regulation of CD44 expression in human prostatic carcinoma cell lines is correlated with DNA hypermethylation.

Author

Verkaik NS, Trapman J, Romijn JC, Van der Kwast TH, and Van Steenbrugge GJ

Subjects

Antimetabolites, Antineoplastic pharmacology, Azacitidine pharmacology, Down-Regulation, Humans, Hyaluronan Receptors genetics, Male, Neoplasm Proteins genetics, Prostatic Neoplasms genetics, RNA, Messenger metabolism, Tumor Cells, Cultured, CpG Islands physiology, DNA Methylation, DNA, Neoplasm metabolism, Hyaluronan Receptors metabolism, Neoplasm Proteins metabolism, Prostatic Neoplasms metabolism

Abstract

Down-regulation of the cell-surface adhesion molecule CD44 has been suggested to play an important role in tumor progression and metastasis of prostate cancer. CD44 is encoded by a gene that contains a CpG-rich region (CpG island) in its 5' regulatory sequence. We tried to assess whether hypermethylation of this region is the mechanism responsible for CD44 transcriptional inactivation. A panel of prostatic-carcinoma cell lines, Du145, LNCaP, PC3, PC346C and TSU, was analyzed for CD44 mRNA and protein expression. Du145, PC3 and TSU were positive for CD44, whereas in LNCaP and PC346C both CD44 mRNA and protein expression was suppressed. Methylation-sensitive restriction-enzyme analysis of genomic DNA showed that, in contrast to the CD44-positive cell lines, the CD44-negative lines were hypermethylated in the CD44 promoter CpG island. Furthermore, treatment of a PC346C culture with the demethylating agent 5-azacytidine resulted in re-expression of CD44 mRNA. It is concluded that hypermethylation of the CD44 5' promoter region is one of the mechanisms by which CD44 expression is down-regulated in prostatic-carcinoma cell lines.

Published

1999

33. Characterization of chromosome 8 aberrations in the prostate cancer cell line LNCaP-FGC and sublines.

Author

König JJ, Teubel W, van Steenbrugge GJ, Romijn JC, and Hagemeijer A

Subjects

Cosmids genetics, Gene Deletion, Gene Dosage, Humans, In Situ Hybridization, Fluorescence, Male, Molecular Biology methods, Tumor Cells, Cultured, Chromosome Aberrations genetics, Chromosomes, Human, Pair 8 genetics, Prostatic Neoplasms genetics

Abstract

In two androgen-dependent (FGC and P70) and two androgen-independent (LNO and R) sublines of the prostate cancer model LNCaP numerical and structural aberrations of chromosome 8 were investigated in detail. The techniques used were whole chromosome paint (WCP) and fluorescence in situ hybridization (FISH) with three cosmid probes mapping to different parts of the p-arm (D8S7 (8p23.3), LPL (8p22) and PLAT (8p11.1)). By WCP all four cell lines showed four copies of chromosome 8 in most cells. However, FISH demonstrated that in all sublines deletions in the 8p region were present. The majority of both FGC and P70 had two copies of cosmids D8S7 and LPL. The cosmid PLAT showed a broader distribution (1-4 copies), especially in P70. Compared with FGC and P70, both LNO and R showed a larger number of copies (3 or 4) of all three cosmid loci. It is discussed that this difference is probably the result of nondisjunction as a reaction to loss of other sequences on 8p, possibly the tumor suppressor gene (TSG) mapping to 8p21. The fact that both sublines LNO and R are androgen-independent raises the possibility of a link between TSG loss on 8p and androgen independence.

Published

1999

34. The human prostate-specific transglutaminase gene (TGM4): genomic organization, tissue-specific expression, and promoter characterization.

Author

Dubbink HJ, de Waal L, van Haperen R, Verkaik NS, Trapman J, and Romijn JC

Subjects

Amino Acid Sequence, Base Sequence, Exons genetics, Genes, Reporter genetics, Humans, Introns genetics, Male, Molecular Sequence Data, Peptidylprolyl Isomerase chemistry, Protein Biosynthesis genetics, Pseudogenes genetics, RNA Splicing genetics, RNA, Messenger metabolism, Sequence Analysis, DNA, Transcription, Genetic genetics, Transfection genetics, Transglutaminases chemistry, Tumor Cells, Cultured, Gene Expression Regulation, Enzymologic genetics, Promoter Regions, Genetic genetics, Prostate enzymology, Transglutaminases genetics

Abstract

Human prostate-specific transglutaminase (hTGP) is a cross-linking enzyme secreted by the prostate. In this study, we performed dot blot analysis of 50 normal human tissues to demonstrate unambiguously the prostate-specific expression of hTGP. Furthermore, we elucidated the genomic organization of the TGM4 gene, the gene encoding hTGP. The structure of this gene displays striking similarity to that of other transglutaminase (TGase) genes. The TGM4 gene spans approximately 35 kb of genomic DNA and consists of 13 exons and 12 introns. The main transcription initiation site is located 52 bp upstream of the translational start codon. A hTGP splice variant of intron 1 was detected. This splice variant contains an in-frame antisense Alu element insertion. The TGM4 promoter was analyzed by sequencing and transfection experiments. At positions -1276 to -563, the promoter harbors a cyclophilin pseudogene with 94% similarity to the cyclophilin A cDNA. Deletion mapping of the TGM4 promoter in the transiently transfected human prostate cancer cell line PC346C showed comparable activity of 2.1-, 1.5-, and 0.5-kb promoter fragments., (Copyright 1998 Academic Press.)

Published

1998

35. Increased calcium oxalate monohydrate crystal binding to injured renal tubular epithelial cells in culture.

Author

Verkoelen CF, van der Boom BG, Houtsmuller AB, Schröder FH, and Romijn JC

Subjects

Animals, Cell Death, Cell Line, Dogs, Microscopy, Confocal, Wound Healing, Calcium Oxalate metabolism, Epithelial Cells metabolism, Epithelial Cells pathology, Kidney Tubules metabolism, Kidney Tubules pathology

Abstract

The retention of crystals in the kidney is considered to be a crucial step in the development of a renal stone. This study demonstrates the time-dependent alterations in the extent of calcium oxalate (CaOx) monohydrate (COM) crystal binding to Madin-Darby canine kidney (MDCK) cells during their growth to confluence and during the healing of wounds made in confluent monolayers. As determined by radiolabeled COM crystal binding studies and confirmed by confocal-scanning laser microscopy, relatively large amounts of crystals (10.4 +/- 0.4 micrograms/cm2) bound to subconfluent cultures that still exhibited a low transepithelial electrical resistance (TER < 400 omega.cm2). The development of junctional integrity, indicated by a high resistance (TER > 1,500 omega.cm2), was followed by a decrease of the crystal binding capacity to almost undetectable low levels (0.13 +/- 0.03 microgram/cm2). Epithelial injury resulted in increased crystal adherence. The highest level of crystal binding was observed 2 days postinjury when the wounds were already morphologically closed but TER was still low. Confocal images showed that during the repair process, crystals selectively adhered to migrating cells at the wound border and to stacked cells at sites were the wounds were closed. After the barrier integrity was restored, crystal binding decreased again to the same low levels as in undamaged controls. These results indicate that, whereas functional MDCK monolayers are largely protected against COM crystal adherence, epithelial injury and the subsequent process of wound healing lead to increased crystal binding.

Published

1998

36. Expression of prostatic factors measured by reverse transcription polymerase chain reaction in human papillomavirus type 18 deoxyribonucleic acid immortalized prostate cell lines.

Author

Weijerman PC, Zhang Y, Shen J, Dubbink HJ, Romijn JC, Peehl DM, and Schröder FH

Subjects

Antigens, Surface analysis, Carboxypeptidases analysis, Cells, Cultured, Glutamate Carboxypeptidase II, Humans, Male, Polymerase Chain Reaction, Prostate cytology, Prostate-Specific Antigen analysis, Receptors, Androgen analysis, Antigens, Surface biosynthesis, Carboxypeptidases biosynthesis, Papillomaviridae genetics, Prostate metabolism, Prostate-Specific Antigen biosynthesis, Receptors, Androgen biosynthesis, Transfection

Abstract

Objectives: To investigate expression of the prostatic markers prostate-specific antigen (PSA), prostate-specific membrane antigen (PSM), and the androgen receptor (AR) after human papillomavirus (HPV) type 18 deoxyribonucleic acid (DNA) transfection and subsequent immortalization of human prostate epithelial cells., Methods: Recently, two human prostate epithelial cell lines were established by HPV transformation: PZ-HPV-7, derived from normal peripheral zone (PZ) tissue, and CA-HPV-10, derived from high Gleason grade adenocarcinoma. Expression of PSA was studied by the reverse transcription polymerase chain reaction (RT-PCR), because in preliminary studies using immunocytochemistry and Northern blotting, no PSA expression was found. PSM was analyzed by RT-PCR and nested RT-PCR. These analyses included primary human prostate cell strains. Furthermore, androgen-supplemented methylthiazol tetrazolium (MTT) growth assays were performed and expression of AR was studied by immunocytochemistry. Prostate carcinoma cell lines LNCaP and PC-346C were included as positive controls and breast carcinoma cell line MCF-7 as a negative control., Results: Both cell lines exhibited low levels of RNA for PSA and PSM in comparison with cell lines LNCaP and PC-346C. AR expression by immunocytochemistry was negative using monoclonal antibody F39.4 and polyclonal antibody SP-197. In an androgen-supplemented environment, growth rates of both HPV immortalized cell lines were not stimulated in contrast to LNCaP., Conclusions: RNA transcripts of PSA and PSM were detected by RT-PCR in HPV immortalized prostate epithelial cell lines PZ-HPV-7 and CA-HPV-10. The expression of prostate-specific markers may further validate the utility of this stepwise transformation model of human prostate carcinogenesis.

Published

1998

37. Cytogenetic analysis of 39 prostate carcinomas and evaluation of short-term tissue culture techniques.

Author

König JJ, Teubel W, Kamst E, Romijn JC, Schröder FH, and Hagemeijer A

Subjects

Carcinoma chemistry, Carcinoma pathology, Cell Division drug effects, Cells, Cultured, Evaluation Studies as Topic, Humans, Immunohistochemistry, Keratins analysis, Male, Prostate-Specific Antigen analysis, Prostatic Neoplasms chemistry, Prostatic Neoplasms pathology, Carcinoma genetics, Culture Techniques methods, Karyotyping methods, Prostatic Neoplasms genetics

Abstract

Karyotypic analysis was performed on 102 prostate cancer specimens which were obtained through radical prostatectomy, transurethral resection, or regional lymph node dissection. Short term tissue culture was applied in all cases. Of the media and growth factors evaluated, F12/DMEM, supplemented with 2% fetal calf serum, insulin, epidermal growth factor, hydrocortisone, and cholera toxin produced the largest increase of in vitro proliferation. Such in vitro cultured cells were all phenotypically acinar epithelial cells, the supposed targets for neoplastic transformation. Stromal cell growth appeared to be completely suppressed. Of the three culture techniques investigated, the method developed in Lund, Sweden, was the most successful: 11/15 cultures yielded metaphases and, in three of these, clonal aberrations were identified. All 39 karyotypes obtained essentially had a 46,XY karyotype with clonal aberrations (eight cases) and/or nonclonal aberrations (30 cases). Clonal structural aberrations involved 2p, 3q, 11p, 17p, and 21q. The clonal numerical aberrations found were: + 8, + dmin, and -Y. The most frequently observed nonclonal aberrations were 8p deletions (five cases) and loss of 6, 7, 8, 15, 17, 18, 21, and/or Y (> or = five cases). In summary, clonal aberrations were observed in 20% of the evaluable PC cell cultures, and nonclonal aberrations in 77%. So, although diploid cells without clonal abnormalities still had a growth advantage, under optimal conditions PC cells were able to proliferate in primary in vitro culture.

Published

1998

38. Specific cytogenetic aberrations in two novel human prostatic cell lines immortalized by human papillomavirus type 18 DNA.

Author

Weijerman PC, van Drunen E, König JJ, Teubel W, Romijn JC, Schröder FH, and Hagemeijer A

Subjects

Chromosome Banding, Genetic Markers, Humans, In Situ Hybridization, Fluorescence, Karyotyping, Male, Ploidies, Transfection, Tumor Cells, Cultured, Cell Line, Transformed, Chromosome Aberrations, DNA, Viral, Papillomaviridae genetics, Prostatic Neoplasms genetics

Abstract

Using chromosome banding and fluorescence in situ hybridization (FISH) with painting probes, sequential cytogenetic analysis was performed of two novel prostate cell lines, PZ-HPV-7 and CA-HPV-10, established by human papillomavirus (HPV) 18 DNA transformation. PZ-HPV-7 originates from a normal diploid prostate epithelial cell strain. PZ-HPV-7 progressed from an initial diploid to a hypertetraploid chromosome number with a relative gain of chromosomes 5 and 20 (7 to 8 copies each). Structural changes were limited; 3p- (2 copies), 3q- (1 copy), and possibly a der(16p;12q). CA-HPV-10 originates from an epithelial cell strain derived from a high-grade human prostate cancer specimen, which showed several karyotypic abnormalities including an extra Y chromosome and double minutes (dmin). In early passage the karyotype of CA-HPV-10 appeared unstable with a decreasing number of cells exhibiting dmin. In late passage the dmin were replaced by a large homogeneously staining region (hsr) on 9p+ marker. The hsr was shown by FISH to be of chromosome 1 origin. The modal number was mainly hypertriploid (72, range 69 to 75). Loss of Y was remarkable (0 to 1 copy). Consistent markers included two copies each of del(1)(q12q31) and der(9)t(1;9)(?;p22), and one der(11)t(4;11) (?;q21). HPV type 18 genomic integration sites were identified on 1p for PZ-HPV-7 and on the 9p+ marker for CA-HPV-10. In conclusion, both PZ-HPV-7 and CA-HPV-10 showed clonal cytogenetic changes. These two cell lines constitute a novel in vitro model to study the mechanisms involved in human prostate carcino-genesis.

Published

1997

39. Orthotopic implantation of human prostate cancer cell lines: a clinically relevant animal model for metastatic prostate cancer.

Author

Rembrink K, Romijn JC, van der Kwast TH, Rübben H, and Schröder FH

Subjects

Animals, Disease Models, Animal, Humans, Immunohistochemistry, Injections, Subcutaneous, Lung Neoplasms metabolism, Lung Neoplasms pathology, Lung Neoplasms secondary, Male, Mice, Mice, Nude, Neoplasm Invasiveness, Prostate pathology, Prostate-Specific Antigen analysis, Receptors, Androgen metabolism, Staining and Labeling, Tumor Cells, Cultured, Cell Transplantation, Prostatic Neoplasms pathology

Abstract

Background: To study the metastatic behavior of human prostate cancer cell lines, orthotopic injection in nude mice was performed., Methods: Local tumor growth, metastasis formation, prostate-specific antigen, and androgen receptor expression were examined., Results: Hormone-independent cell lines (PC-3, PC-3-125-IL, and TSU-Pr1) were highly tumorigenic and had a higher rate of lymph node metastasis after orthotopic than after subcutaneous implantation. PC-3 cell lines also consistently metastasized to the lungs. The androgen-sensitive LNCaP cell line showed local growth in 7 of 10, and lymph node metastasis in 4 animals. Significant serum PSA levels and strong receptor expression in primary and metastatic tumor tissues were observed., Conclusions: These results demonstrates that orthotopic implantation of human prostate cancer cell lines, including LNCaP, reproducibly leads to metastasis formation in nude mice.

Published

1997

40. Cell cultures and nephrolithiasis.

Author

Verkoelen CF, van der Boom BG, Schröder FH, and Romijn JC

Subjects

Animals, Calculi metabolism, Cells, Cultured, Crystallization, Humans, Kidney Calculi physiopathology, Models, Theoretical, Calculi chemistry, Kidney Calculi etiology, Kidney Tubules cytology

Abstract

While the physical chemistry of stone formation has been intensively studied during the last decade, it has become clear that the pathophysiology of renal stone disease cannot be explained by crystallization processes only. In recent years, evidence has emerged that the cells lining the renal tubules can have an active role in creating the conditions under which stones may develop. Since it is difficult to study these mechanisms in vivo, cultured renal tubular cells have become increasingly popular for the study of physiological and cell biological processes that are possibly linked to stone disease. In this paper, we discuss the possible contribution of cellular processes such as transepithelial oxalate transport and crystal--cell interaction to the formation of renal stones. Experimental studies that have been performed with cultured renal cells to elucidate the mechanisms involved in these processes will be summarized.

Published

1997

41. Stromal inhibition of epithelial cell growth in the prostate; overview of an experimental study.

Author

Kooistra A, Romijn JC, and Schröder FH

Subjects

Antibodies, Blocking pharmacology, Cell Division physiology, Cell Line, Cells, Cultured, Culture Media, Conditioned, Epithelial Cells, Epithelium physiology, Growth Inhibitors physiology, Humans, Male, Neutralization Tests, Prostate physiology, Prostatic Hyperplasia pathology, Prostatic Hyperplasia physiopathology, Prostatic Neoplasms pathology, Prostatic Neoplasms physiopathology, Transforming Growth Factor beta antagonists & inhibitors, Transforming Growth Factor beta physiology, Tumor Cells, Cultured, Prostate cytology

Abstract

The paracrine influence of prostatic stroma on the proliferation of prostatic epithelial cells was investigated. Using a double-layer soft agar assay it was demonstrated that stromal cells from the human prostate inhibit the anchorage-independent growth of the prostatic tumor epithelial cell lines PC-3 and LNCaP. Anchorage-dependent growth was inhibited too as was shown in the semi-automated colorimetric MTT test performed on multiwell plates. Antiproliferative activity was mediated by a diffusible factor in the stromal cell conditioned medium and was found to be produced specifically by prostatic stromal cells. Although the putative inhibiting factor shared some properties with transforming growth factor beta (TGF-beta) evidence is presented that the factor is different from this well-known inhibitor of epithelial cell growth. Absence of TGF-beta activity was shown by the lack of inhibitory response of the TGF-beta-sensitive mink lung cell line CCL-64 to prostate stromal cell conditioned medium and to concentrated partially purified preparations of the inhibitor. Furthermore, neutralizing antibodies against TGF-beta 1 or TGF-beta 2 did not cause a decline in the level of PC-3 growth inhibition caused by partially purified inhibitor. It is concluded that the prostate stroma-derived factor may be a novel growth inhibitor different from any of the currently described inhibiting factors.

Published

1997

42. Does urinary oxalate interfere with the inhibitory role of glycosaminoglycans and semisynthetic sulfated polysaccharides in calcium oxalate crystallization?

Author

Cao LC, Deng G, Boevé ER, Romijn JC, de Bruijn WC, Verkoelen CF, and Schröder FH

Subjects

Calcium Oxalate urine, Crystallization, Glycosaminoglycans pharmacology, Hydrogen-Ion Concentration, Polysaccharides pharmacology, Software, Urinary Calculi urine, Calcium Oxalate chemistry, Glycosaminoglycans metabolism, Oxalates urine, Polysaccharides metabolism

Abstract

Objectives: Previously it was shown that the polysaccharide G872 in vitro strongly inhibits calcium oxalate monohydrate crystallization processes. However, when rats on a stone-inducing diet of ethylene glycol plus vitamin D3 are given this polysaccharide, no changes in the urine capacity for crystallization inhibition were found. We investigated here how the inhibitory action of polysaccharides changes under high oxalate conditions, as they exist in the stone inducing diet., Methods: Calcium oxalate monohydrate (COM) crystals were incubated in a series of 0.05 M PBS buffers containing polysaccharides with increasing oxalate concentrations (0-0.4 mmol/l). The coated crystals were collected, washed and resuspended in an artificial urine. We then measured the zeta potential of the crystals, using a Coulter DELSA 440, and the initial rates for crystal growth and agglomeration, using the Coulter Multisizer II., Results: Addition of oxalate to the medium shifts the negative zeta potential distribution of COM crystals coated by polysaccharides in positive direction. Particle size analysis demonstrated that the initial rates of COM crystal growth and agglomeration responding to oxalate concentration changes (0.1-->0.4 mmol/l) in the presence of G872 (0.2 mg/l) are approximately 2.5 times faster than that in the absence of G872., Conclusions: Oxalate interferes with the binding of polysaccharides to crystals. This can be envisioned to occur through changes in the crystal surface properties or by induction of functional and secondary structural changes of urinary macromolecular inhibitors such as GAGs, resulting in a decrease of their inhibitory activity against COM crystallization. Thus, in urine, a high oxalate may increase the rate of crystallization both by increasing the supersaturation and by decreasing the inhibitory potential of the urine.

Published

1997

43. Decreased levels of topoisomerase II alpha in human renal cell carcinoma lines resistant to etoposide.

Author

Scheltema JM, Romijn JC, van Steenbrugge GJ, Beck WT, Schröder FH, and Mickisch GH

Subjects

Antigens, Neoplasm, Antineoplastic Agents pharmacology, DNA Methylation, DNA-Binding Proteins, Doxorubicin pharmacology, Drug Resistance, Multiple, Drug Resistance, Neoplasm, Gene Expression drug effects, Humans, Polymorphism, Single-Stranded Conformational, RNA, Messenger genetics, RNA, Neoplasm genetics, Tumor Cells, Cultured, Vinblastine pharmacology, Carcinoma, Renal Cell enzymology, DNA Topoisomerases, Type II metabolism, Etoposide pharmacology, Isoenzymes metabolism, Kidney Neoplasms enzymology

Abstract

Renal cell carcinoma (RCC) displays strong resistance against many chemotherapeutic drugs. Overexpression of P-glycoprotein (Pgp) appears to be part of this resistance. The involvement of another resistance mechanism, involving the decreased activity of DNA topoisomerase II (topoII), remains uncertain. By culturing the human RCC lines RC2 and RC21 in the presence of increasing concentrations of etoposide, we derived the variant sublines RC2E, RC21A and RC21E, that had acquired approximately 30-, 60- and 90-fold resistance to this drug respectively. RC2E, RC21A and RC21E were approximately 50-, 5- and 400-fold cross-resistant to doxorubicin respectively. RC2E and RC21E also showed cross-resistance (approximately 200- and 3500-fold respectively) to vinblastine. Quantitative differences in MDR1 and Pgp expression (elevated in RC2E and RC21E) and topoII alpha (reduced in RC21E and RC21A) were demonstrated using Western blotting and the reverse transcriptase/polymerase chain reaction. Decreased amounts of topoII alpha were reflected in a reduced activity of RC21A and RC21E as measured by unknotting phage P4 DNA. Qualitative changes of the topoII alpha gene, such as point mutations in the motif B/DNBS and DNA-binding regions, or differences in methylation status of the promoter gene of RC21E, were not found. These cell lines represent a model of a solid tumor in which overexpression of Pgp, a combination of increased Pgp and decreased topoII alpha, and a decrease of topoII alpha are represented.

Published

1997

44. Clinical usefulness of RT-PCR detection of hematogenous prostate cancer spread.

Author

Verkaik NS, Schröder FH, and Romijn JC

Subjects

Carboxypeptidases blood, Glutamate Carboxypeptidase II, Humans, Male, Prostate-Specific Antigen blood, Prostatic Neoplasms blood, Antigens, Surface, Biomarkers, Tumor blood, Neoplastic Cells, Circulating, Polymerase Chain Reaction, Prostatic Neoplasms pathology

Abstract

Understaging is commonly associated with therapeutic failure of surgical intervention in apparently localized prostate cancers. Methods that specifically detect prostate cancer cells in the circulation may be able to identify metastatic cancers and thus aid in the selection of the most adequate therapy. The high sensitivity and specificity of the reverse transcriptase-polymerase chain reaction (RT-PCR) encouraged various groups to investigate the mRNA expression of prostate-specific markers in the peripheral blood of patients with prostate cancer. However, probably due to methodological differences, many contradictory results have been obtained with the markers studied so far: prostate-specific antigen (PSA) and prostate-specific membrane antigen (PSM). For this reason, clinical decisions should not be based yet on RT-PCR results. Future research and long-term follow-up on the patients may point out whether RT-PCR assays, following appropriate standardization, will have an additive value in prostate cancer staging and in prediction of tumor progression.

Published

1997

45. Development of seven new human prostate tumor xenograft models and their histopathological characterization.

Author

van Weerden WM, de Ridder CM, Verdaasdonk CL, Romijn JC, van der Kwast TH, Schröder FH, and van Steenbrugge GJ

Subjects

Animals, Cell Division, DNA, Neoplasm chemistry, Female, Humans, Male, Mice, Mice, Inbred BALB C, Mice, Nude, Neoplasm Transplantation methods, Ploidies, Prostatic Neoplasms genetics, Transplantation, Heterologous, Tumor Cells, Cultured, Disease Models, Animal, Prostatic Neoplasms pathology

Abstract

Seven human prostate tumor models were established by transplanting tumor fragments in NMRI athymic nude mice. Once established, the tumors were serially transplantable in both NMRI and BALB/c nude mice. The xenografts originated from primary prostatic carcinomas (prostatectomy specimens), transurethral resection material, and metastatic lesions (pelvic lymph nodes and scrotal skin). Histological examination revealed that, in the course of several mouse passages (8 to 23), tumors retained their resemblance to the original patient material. The PC-295, PC-310, PC-329, and PC-346 tumors are dependent on androgens for their growth. The PC-324, PC-339, and PC-374 tumors are androgen independent, although growth of PC-374 tumors still seemed androgen sensitive. All tumors are diploid, except for the PC-374, which is tetraploid. The diploid PC-295 tumor has an additional small population of tetraploid cells. All xenografts displayed a heterogeneous expression pattern of the androgen receptor except for the PC-324 and PC-339 tumors in which the androgen receptor could not be detected. Prostatic acid phosphatase and prostate-specific antigen were retained during serial transplantation in all tumors but the PC-324 and PC-339. This panel of permanent human prostate tumor models comprises tumors representing both the androgen-dependent and -independent stages of human prostate cancer with various degrees of differentiation and, therefore, is of great value for the study of many aspects of growth and progression of human prostate cancer.

Published

1996

46. Gain and loss of chromosomes 1, 7, 8, 10, 18, and Y in 46 prostate cancers.

Author

König JJ, Teubel W, Romijn JC, Schröder FH, and Hagemeijer A

Subjects

Aged, Aged, 80 and over, Chromosomes, Human, Pair 1, Chromosomes, Human, Pair 10, Chromosomes, Human, Pair 18, Chromosomes, Human, Pair 7, Chromosomes, Human, Pair 8, DNA, Neoplasm genetics, Flow Cytometry, Humans, In Situ Hybridization, Fluorescence, Male, Middle Aged, Neoplasm Staging, Prostatic Hyperplasia genetics, Prostatic Neoplasms pathology, Y Chromosome, Aneuploidy, Prostatic Neoplasms genetics

Abstract

Fluorescence in situ hybridization (FISH) with centromere probes was used to investigate numerical aberrations of chromosomes 1, 7, 8, 10, 18, and Y in 46 prostate carcinoma (PC) and 11 benign prostatic hyperplasia (BPH) samples. None of the benign specimens showed any chromosomal aberration. Forty-one of 46 PC specimens showed numerical aberrations of one or more chromosomes. All investigated chromosomes showed numerical aberrations in at least 30% of the specimens, gain being more frequent than loss. Comparison of DNA flow cytometry (FCM) and FISH results showed that not only aneuploid tumors but also most diploid tumors harbored numerical chromosome aberrations. Chromosome 10 was the most frequently gained (65%), and Y the most frequently lost chromosome (14%). Nonmetastatic and metastatic tumors differed significantly (P < .05) in the number of copies for chromosomes 7, 8, and 10, but not for 1, 18, and Y. These results suggest strongly that gains of chromosomes 7, 8, and 10 are involved in PC progression.

Published

1996

47. Tissue specific and androgen-regulated expression of human prostate-specific transglutaminase.

Author

Dubbink HJ, Verkaik NS, Faber PW, Trapman J, Schröder FH, and Romijn JC

Subjects

Amino Acid Sequence, Animals, Base Sequence, Chromosome Mapping, Chromosomes, Human, Pair 3 genetics, Cloning, Molecular, Cricetinae, DNA Probes genetics, DNA, Complementary genetics, Female, Gene Expression Regulation, Enzymologic, Humans, Hybrid Cells, Male, Mice, Molecular Sequence Data, Prostatic Neoplasms enzymology, Prostatic Neoplasms genetics, Sequence Homology, Amino Acid, Tissue Distribution, Transglutaminases genetics, Tumor Cells, Cultured, Androgens metabolism, Prostate enzymology, Transglutaminases metabolism

Abstract

Transglutaminases (TGases) are calcium-dependent enzymes catalysing the post-translational cross-linking of proteins. In the prostate at least two TGases are present, the ubiquitously expressed tissue-type TGase (TGC), and a prostate-restricted TGase (TGP). This paper deals with the molecular cloning and characterization of the cDNA encoding the human prostate TGase (hTGP). For this purpose we have screened a human prostate cDNA library with a probe from the active-site region of TGC. The largest isolated cDNA contained an open reading frame encoding a protein of 684 amino acids with a predicted molecular mass of 77 kDa as confirmed by in vitro transcription-translation and subsequent SDS/PAGE. The hTGP gene was tissue-specifically expressed in the prostate, yielding an mRNA of approx. 3.5 kb. Furthermore, a 3-fold androgen-induced upregulation of hTGP mRNA expression has been demonstrated in the recently developed human prostate cancer cell line, PC346C. Other well established human prostate cancer cell lines, LNCaP and PC-3, showed no detectable hTGP mRNA expression on a Northern bolt. The gene coding for prostate TGase was assigned to chromosome 3.

Published

1996

48. Crystal-cell interaction inhibition by polysaccharides.

Author

Verkoelen CF, Romijn JC, Cao LC, Boevé ER, De Bruijn WC, and Schröder FH

Subjects

Analysis of Variance, Animals, Cells, Cultured, Crystallization, Dogs, Surface Properties, Calcium Oxalate, Kidney cytology, Kidney drug effects, Polysaccharides pharmacology

Abstract

Purpose: We studied the effect of polysaccharides on interactions between calcium oxalate monohydrate (COM) crystals and cultured renal cells., Materials and Methods: Monolayers of Madin-Darby canine kidney (MDCK) cells were incubated with radiolabeled crystals in the presence of various concentrations of natural glycosaminoglycans (GAGs) and semisynthetic polysaccharides (SSPs)., Results: While most GAGs were found to have relatively little effect, SSPs (SP54, G871 and G872) were potent inhibitors of crystal-cell association. Pretreatment of crystals, but not of cells, was similarly effective, suggesting polysaccharide-induced modification of crystal surface properties., Conclusions: This result further supports the idea that SSPs, and especially G872, are of potential interest for treatment of recurrent stone disease.

Published

1996

49. Lectin-cytochemistry of experimental rat nephrolithiasis.

Author

de Bruijn WC, de Water R, Boevé ER, van Run PR, Vermaire PJ, van Miert PP, Romijn JC, Verkoelen CF, Cao LC, and Schröder FH

Subjects

Animals, Crystallization, Immunohistochemistry, Kidney ultrastructure, Kidney Calculi ultrastructure, Osteopontin, Polysaccharides pharmacology, Rats, Sialoglycoproteins genetics, Tissue Embedding, Kidney chemistry, Kidney Calculi metabolism, Lectins metabolism, Sialoglycoproteins analysis

Abstract

Lectin reactivity in epithelial apical cell coats of normal rat kidneys was compared to that from animals subjected to crystal inducing diets (CID). The aim was to see whether the absence of lectin reactivity in cell coats is related to intratubular calcium oxalate crystal retention. In normal rat kidneys, after a pre-embedding procedure, it was observed that at the ultrastructural level, reactivity was present but that the lectin specificity for the various parts of the nephron might have to be reconsidered. There was heterogeneity between the epithelial cells with respect to the presence of coat material in the tubular cell apices. Tubular epithelial cell apices from CID rats showed no obvious changes in lectin reactivity pattern. Lectin reactivity was present at the periphery of intratubular crystals but undetectable at true crystal attachment sites or reduced at cell apices in the vicinity of recently attached crystals or agglomerates. After a post-embedding reaction procedure, wheat-germ agglutinin (WGA)-lectin reactivity confirmed the presence of coat material in the cleft between cell apex and retained crystal at crystal-attachment sites. The WGA/Au-10 nm reaction products were also seen inside epithelial cells. WGA/Au-10 nm reaction products mark a crystal matrix component inside intratubular and retained crystals. A similar matrix was also marked by an alpha-osteopontin (alpha OPN/Au-10 nm) reaction product.

Published

1996

50. Zeta potential measurement and particle size analysis for a better understanding of urinary inhibitors of calcium oxalate crystallization.

Author

Cao LC, Deng G, Boevé ER, de Bruijn WC, de Water R, Verkoelen CF, Romijn JC, and Schröder FH

Subjects

Cetylpyridinium pharmacology, Crystallization, Humans, Particle Size, Polysaccharides pharmacology, Urine physiology, Calcium Oxalate chemistry, Kidney Calculi prevention & control, Urine chemistry

Abstract

To better understand urinary inhibitors of calcium oxalate crystallization, both zeta potential measurement and particle size analysis were chosen to illustrate: (1) the potential therapeutic efficacy of G872, a semi-synthetic sulfated polysaccharide, in stone prevention; and (2) the relative contribution of various urinary fractions ¿e.g., ultrafiltered urine (UFU), Tamm-Horsfall protein (THP), urinary polyanions precipitated with cetylpyridinium chloride (CPC), urinary macromolecular substances with different concentration ratios (UMS10,50,90 and UMS'10,50,90) and THP-free urine (THPFU)¿ to total urinary inhibitory activity. The results showed: (1) addition of G872 significantly enhances urinary inhibitory activity and negative zeta potential values; (2) re-addition of the CPC to UFU completely restores urinary inhibitory activity; and (3) artificial urines prepared by mixing UMS'10,50,90 from THPFU with UFU differed in inhibitory activity from that prepared by mixing UMS10,50,90 from a pooled normal urine with UFU. Based on these experimental results, the following speculations can be made: (1) normal human urines are considered to be a protective colloidal system; (2) urinary inhibitory activity originates mainly from CPC and/or UMS; (3) normal THP is a protective material to maintain urinary inhibitory activity; and (4) mutual interaction between urinary inhibitors may change the total urinary inhibitory activity.

Published

1996