Your search keyword '"Vleminckx, K."' showing total 4 results

1. Effect of oncogene transfection or passage in vivo on malignant phenotypes of rat2 cells

Author

Fm, Roy, Peter Coopman, Suffys P, Liebaut G, Vleminckx K, Gao J, Ch, Dragonetti, Fiers W, and Mm, Mareel

Subjects

Cell Transformation, Neoplastic, Genes, ras, Phenotype, Animals, DNA, Oncogenes, Cosmids, Embryo, Mammalian, Transfection, Thymidine Kinase, Cell Division, Cell Line, Rats

Abstract

Rat2 cells are thymidine kinase-deficient derivatives from the immortalized rat embryo cell line Rat1. They show no phenotypic correlates of malignancy in vitro and produce tumors in syngeneic Fischer rats after long latency periods. We have investigated how transfection with oncogenes would alter the in vitro and in vivo behavior of Rat2 cells. Thus we have manipulated Rat2 cultures in various ways. The cell lines obtained were categorized as parental, in vitro subclones, untransfected in vivo derivatives, non-oncogene (neor and tk) transfectants, oncogene (mutated c-Ha-ras, polyoma middle-T, FBR v-gag-fos-fox) transfectants, and in vivo derivatives of transfectants. They were tested in vitro for morphotype, colony formation in soft agar, growth in organ culture, invasion in organ culture, and in vivo for latency period of tumor formation, tumor growth rate, invasiveness, and metastasis. Differences between the consequences of various manipulations were found in the number of malignancy-related phenotypic alterations. The following trend could be deduced from our data: induction of invasiveness in organ culture by all manipulations; morphotypic transformation and shortening of tumor-latency period by all oncogene transfections and by passage with tumor formation in vivo; growth in organ culture and increased tumor growth rate in vivo by transfection with ras-, or fos-oncogenes and by passage in vivo. Metastatic capability (present in parental Rat2 cell tumors) and colony formation in soft agar (absent in Rat2 cells) were not affected by the present manipulations. We concluded that differences between the oncogene-transfectants and the untransfected in vivo derivatives do not lie in the expression of malignancy-related phenotypes but in the time needed to acquire them.

Published

1989

2. Overlevingspensioen en/of arbeid: noden en behoeften van weduwen

Author

Koen Ponnet, Dimitri Mortelmans, Paul Peter Vermeiren, and Vleminckx, K.

Subjects

Sociology

3. Proffered papers and posters presented at the Sixth International Symposium on Hereditary Breast and Ovarian Cancer—BRCA: Challenges and Opportunities : Presented by the Hereditary Breast and Ovarian Cancer Foundation in collaboration with the Program in Cancer Genetics, McGill University; Centre Mont-Royal, Montreal, QC; 10–13 May 2016

Author

Starita L, Islam M, Fields S, Parvin J, Shendure J, Vierstraete J, Willaert A, Vleminckx K, Vermassen P, Pieters L, Coucke P, Vral A, Claes K, and Chalas E

4. Mechanism underlying synergic activation of tyrosinase promoter by MITF and IRF4

Author

Song, J., Liu, X., Li, J., Liu, H., Peng, Z., Liu, Y., Mei, L., He, C., Cai, X., Hongsheng Chen, Vleminckx, K., and Feng, Y.

Subjects

EXPRESSION, TYR, MITF, integumentary system, MUTATIONS, EUROPEANS, EPITHELIUM, Biology and Life Sciences, MELANOMA, synergy effects, IRF4, MICROPHTHALMIA TRANSCRIPTION FACTOR, Medicine and Health Sciences, GENETIC-DETERMINANTS, PIGMENTATION, transcriptional activation, WAARDENBURG SYNDROME TYPE-2, IN-VIVO

Abstract

Background: The transcription factor interferon regulatory factor 4 (IRF4) was identified to be involved in human pigmentation by genome-wide association studies (GWASs). The rs12203592-[T/C], which is located in intron 4 of IRF4, shows the strongest link to these pigmentation phenotypes including freckling, sun sensitivity, eye and hair color. Previous studies indicated a functional cooperation of IRF4 with Microphthalmia-associated transcription factor (MITF), a causing gene of Waardenburg syndrome (WS), to synergistically trans-activate Tyrosinase (TYR). However, the underlying mechanism is still unknown. Methods: To investigate the importance of DNA binding in the synergic effect of IRF4. Reporter plasmids with mutant TYR promoters was generated to locate the IRF4 DNA binding sites in the Tyrosinase minimal promoter. By building MITF and IRF4 truncated mutations plasmids, the necessary regions of the synergy functions of these two proteins were also located. Results: The cooperative effect between MITF and IRF4 was specific for TYR promoter. The DNA-binding of IRF4 was critical for the synergic function. IRF4 DNA binding sites in TYR promoter were identified. The Trans-activation domains in IRF4 (aa134-207, aa300-420) were both important for the synergic function, whereas the auto-mask domain (aa207-300) appeared to mask the synergic effect. Mutational analysis in MITF indicated that both DNA-binding and transcriptional activation domains were both required for this synergic effect. Conclusions: Here we showed that IRF4 potently synergized with MITF to activate the TYR promoter, which was dependent on DNA binding of IRF4. The synergic domains in both IRF4 and MITF were identified by mutational analysis. This identification of IRF4 as a partner for MITF in regulation of TYR may provide an important molecular function for IRF4 in the genesis of melanocytes and the pathogenic mechanism in WS.