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12. Intrauterine instillation of diluted seminal plasma at oocyte pick-up does not increase the IVF pregnancy rate: a double-blind, placebo controlled, randomized study

Author

von Wolff, M., Rösner, S., Germeyer, A., Jauckus, J., Griesinger, G., Strowitzki, T., von Wolff, M., Rösner, S., Germeyer, A., Jauckus, J., Griesinger, G., and Strowitzki, T.

Abstract

STUDY QUESTION Does intrauterine application of diluted seminal plasma (SP) at the time of ovum pick-up improve the pregnancy rate by ≥14% in IVF treatment? SUMMARY ANSWER Intrauterine instillation of diluted SP at the time of ovum pick-up is unlikely to increase the pregnancy rate by ≥14% in IVF. WHAT IS KNOWN ALREADY SP modulates endometrial function, and sexual intercourse around the time of embryo transfer has been suggested to increase the likelihood of pregnancy. A previous randomized double-blind pilot study demonstrated a strong trend towards increased pregnancy rates following the intracervical application of undiluted SP. As this study was not conclusive and as the finding could have been confounded by sexual intercourse, the intrauterine application of diluted SP was investigated in the present trial. STUDY DESIGN, SIZE, DURATION A single-centre, prospective, double-blind, placebo-controlled, randomized, superiority trial on women undergoing IVF was conducted from April 2007 until February 2012 at the University Department of Gynaecological Endocrinology and Reproductive Medicine, Heidelberg, Germany. PARTICIPANTS/MATERIALS, SETTING, METHODS The study was powered to detect an 14% increase in the clinical pregnancy rate and two sequential tests were planned using the Pocock spending function. At the first interim analysis, 279 women had been randomly assigned to intrauterine diluted SP (20% SP in saline from the patients' partner) (n = 138) or placebo (n = 141) at the time of ovum pick-up. MAIN RESULTS AND THE ROLE OF CHANCE The clinical pregnancy rate per randomized patient was 37/138 (26.8%) in the SP group and 41/141 (29.1%) in the placebo group (difference: −2.3%, 95% confidence interval of the difference: −12.7 to +8.2%; P = 0.69). The live birth rate per randomized patient was 28/138 (20.3%) in the SP group and 33/141 (23.4%) in the placebo group (difference: −3.1%, 95% confidence interval of the difference: −12.7 to +6.6%; P = 0.56). It was decided

Published
2017

13. Endometriosis, endometrium, implantation and fallopian tube

Author

Tan, C. W., primary, Lee, Y. H., additional, Choolani, M., additional, Tan, H. H., additional, Griffith, L., additional, Chan, J., additional, Chuang, P. C., additional, Wu, M. H., additional, Lin, Y. J., additional, Tsai, S. J., additional, Rahmati, M., additional, Petitbarat, M., additional, Dubanchet, S., additional, Bensussan, A., additional, Chaouat, G., additional, Ledee, N., additional, Bissonnette, L., additional, Haouzi, D., additional, Monzo, C., additional, Traver, S., additional, Bringer, S., additional, Faidherbe, J., additional, Perrochia, H., additional, Ait-Ahmed, O., additional, Dechaud, H., additional, Hamamah, S., additional, Ibrahim, M. G., additional, de Arellano, M. L. B., additional, Sachtleben, M., additional, Chiantera, V., additional, Frangini, S., additional, Younes, S., additional, Schneider, A., additional, Plendl, J., additional, Mechsner, S., additional, Ono, M., additional, Hamai, H., additional, Chikawa, A., additional, Teramura, S., additional, Takata, R., additional, Sugimoto, T., additional, Iwahashi, K., additional, Ohhama, N., additional, Nakahira, R., additional, Shigeta, M., additional, Park, I. H., additional, Lee, K. H., additional, Sun, H. G., additional, Kim, S. G., additional, Lee, J. H., additional, Kim, Y. Y., additional, Kim, H. J., additional, Jeon, G. H., additional, Kim, C. M., additional, Bocca, S., additional, Wang, H., additional, Anderson, S., additional, Yu, L., additional, Horcajadas, J., additional, Oehninger, S., additional, Bastu, E., additional, Mutlu, M. F., additional, Celik, C., additional, Yasa, C., additional, Dural, O., additional, Buyru, F., additional, Quintana, F., additional, Cobo, A., additional, Remohi, J., additional, Ferrando, M., additional, Matorras, R., additional, Bermejo, A., additional, Iglesias, C., additional, Cerrillo, M., additional, Ruiz, M., additional, Blesa, D., additional, Simon, C., additional, Garcia-Velasco, J. A., additional, Chamie, L., additional, Ribeiro, D. M. F., additional, Riboldi, M., additional, Pereira, R., additional, Rosa, M. B., additional, Gomes, C., additional, de Mello, P. H., additional, Fettback, P., additional, Domingues, T., additional, Cambiaghi, A., additional, Soares, A. C. P., additional, Kimati, C., additional, Motta, E. L. A., additional, Serafini, P., additional, Hapangama, D. K., additional, Valentijn, A. J., additional, Al-Lamee, H., additional, Palial, K., additional, Drury, J. A., additional, von Zglinicki, T., additional, Saretzki, G., additional, Gargett, C. E., additional, Liao, C. Y., additional, Sung, Y. J., additional, Li, H. Y., additional, Morotti, M., additional, Remorgida, V., additional, Venturini, P. L., additional, Ferrero, S., additional, Nabeta, M., additional, Iki, A., additional, Hashimoto, H., additional, Koizumi, M., additional, Matsubara, Y., additional, Hamada, K., additional, Fujioka, T., additional, Matsubara, K., additional, Kusanagi, Y., additional, Nawa, A., additional, Zanatta, A., additional, da Rocha, A. M., additional, Guerra, J. L., additional, Cogliati, B., additional, Bianchi, P. d. M., additional, Prieto, B., additional, Exposito, A., additional, Mendoza, R., additional, Rabanal, A., additional, Bedaiwy, M., additional, Yi, L., additional, Dahoud, W., additional, Liu, J., additional, Hurd, W., additional, Falcone, T., additional, Biscotti, C., additional, Mesiano, S., additional, Sugiyama, R., additional, Nakagawa, K., additional, Nishi, Y., additional, Kuribayashi, Y., additional, Akira, S., additional, Germeyer, A., additional, Rosner, S., additional, Jauckus, J., additional, Strowitzki, T., additional, von Wolff, M., additional, Khan, K. N., additional, Kitajima, M., additional, Fujishita, A., additional, Nakashima, M., additional, Masuzaki, H., additional, Kajihara, T., additional, Ishihara, O., additional, Brosens, J., additional, Vezmar, K., additional, Savournin, V., additional, Balet, R., additional, Loh, S. F., additional, Tannenbaum, S. R., additional, Chan, J. K. Y., additional, Scarella, A., additional, Chamy, V., additional, Devoto, L., additional, Abrao, M., additional, Sovino, H., additional, Krasnopolskaya, K., additional, Popov, A., additional, Kabanova, D., additional, Beketova, A., additional, Ivakhnenko, V., additional, Shohayeb, A., additional, Wahba, A., additional, Abousetta, A., additional, al-inany, H., additional, El Daly, A., additional, Zayed, M., additional, Kvaskoff, M., additional, Han, J., additional, Missmer, S. A., additional, Navarro, P., additional, Meola, J., additional, Ribas, C. P., additional, Paz, C. P., additional, Ferriani, R. A., additional, Donabela, F. C., additional, Tafi, E., additional, Maggiore, U. L. R., additional, Scala, C., additional, Hackl, J., additional, Strehl, J., additional, Wachter, D., additional, Dittrich, R., additional, Cupisti, S., additional, Hildebrandt, T., additional, Lotz, L., additional, Attig, M., additional, Hoffmann, I., additional, Renner, S., additional, Hartmann, A., additional, Beckmann, M. W., additional, Urquiza, F., additional, Ferrer, C., additional, Incera, E., additional, Azpiroz, A., additional, Junovich, G., additional, Pappalardo, C., additional, Guerrero, G., additional, Pasqualini, S., additional, Gutierrez, G., additional, Corti, L., additional, Sanchez, A. M., additional, Bordignon, P. P., additional, Santambrogio, P., additional, Levi, S., additional, Persico, P., additional, Vigano, P., additional, Papaleo, E., additional, Ferrari, S., additional, Candiani, M., additional, van der Houwen, L. E. E., additional, Schreurs, A. M. F., additional, Lambalk, C. B., additional, Schats, R., additional, Hompes, P. G. A., additional, Mijatovic, V., additional, Xu, S. Y., additional, Li, J., additional, Chen, X. Y., additional, Chen, S. Q., additional, Guo, L. Y., additional, Mathew, D., additional, Nunes, Q., additional, Lane, B., additional, Fernig, D., additional, Hapangama, D., additional, Lind, T., additional, Hammarstrom, M., additional, Golmann, D., additional, Rodriguez-Wallberg, K., additional, Hestiantoro, A., additional, Cakra, A., additional, Aulia, A., additional, Al-Inany, H., additional, Houston, B., additional, Farquhar, C., additional, Tagliaferri, V., additional, Gagliano, D., additional, Immediata, V., additional, Tartaglia, C., additional, Zumpano, A., additional, Campagna, G., additional, Lanzone, A., additional, Guido, M., additional, Matsuzaki, S., additional, Darcha, C., additional, Botchorishvili, R., additional, Pouly, J. L., additional, Mage, G., additional, Canis, M., additional, Shivhare, S. B., additional, Bulmer, J. N., additional, Innes, B. A., additional, Lash, G. E., additional, de Graaff, A. A., additional, Zandstra, H., additional, Smits, L. J., additional, Van Beek, J. J., additional, Dunselman, G. A. J., additional, Bozdag, G., additional, Calis, P. T., additional, Demiralp, D. O., additional, Ayhan, B., additional, Igci, N., additional, Yarali, H., additional, Acar, N., additional, Er, H., additional, Ozmen, A., additional, Ustunel, I., additional, Korgun, E. T., additional, Kuroda, K., additional, Kuroda, M., additional, Arakawa, A., additional, Kitade, M., additional, Brosens, A. I., additional, Brosens, J. J., additional, Takeda, S., additional, and Yao, T., additional

Published
2013
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16. POSTER VIEWING SESSION - ENDOMETRIOSIS, ENDOMETRIUM, IMPLANTATION AND FALLOPIAN TUBE

Author

Palial, K. K., primary, Drury, J., additional, Heathcote, L., additional, Valentijin, A., additional, Farquharson, R. G., additional, Gazvani, R., additional, Rudland, P. S., additional, Hapangama, D. K., additional, Celik, N., additional, Celik, O., additional, Aktan, E., additional, Ozerol, E., additional, Celik, E., additional, Bozkurt, K., additional, Paran, H., additional, Hascalik, S., additional, Ozerol, I., additional, Arase, T., additional, Maruyama, T., additional, Uchida, H., additional, Miyazaki, K., additional, Oda, H., additional, Uchida-Nishikawa, S., additional, Kagami, M., additional, Yamazaki, A., additional, Tamaki, K., additional, Yoshimura, Y., additional, De Vos, M., additional, Ortega, C., additional, Smitz, J., additional, Van Vaerenbergh, I., additional, Bourgain, C., additional, Devroey, P., additional, Luciano, D., additional, Exacoustos, C., additional, Zupi, E., additional, Luciano, A. A., additional, Arduini, D., additional, Palomino, W. A., additional, Argandona, F., additional, Kohen, P., additional, Azua, R., additional, Scarella, A., additional, Devoto, L., additional, McKinnon, B., additional, Bersinger, N. A., additional, Mueller, M. D., additional, Bonavita, M., additional, Mattila, M., additional, Ferreira, F. P., additional, Maia-Filho, V., additional, Rocha, A. M., additional, Serafini, P., additional, Motta, E. L. A., additional, Kim, H., additional, Kim, C. H., additional, You, R. M., additional, Nah, H. Y., additional, Lee, J. W., additional, Kang, H. J., additional, Kang, B. M., additional, Letur - Koenirsch, H., additional, Haouzi, D., additional, Olivennes, F., additional, Rouleau, C., additional, Cohen-Bacri, P., additional, Dechaud, H., additional, Hamamah, S., additional, D'Hooghe, T., additional, Hummelshoj, L., additional, Dunselman, G. A. J., additional, Dirksen, C. D., additional, EndoCost Consortium, W. E. R. F., additional, Simoens, S., additional, Novembri, R., additional, Luisi, S., additional, Carrarelli, P., additional, Rocha, A. L. L., additional, Toti, P., additional, Reis, F. M., additional, Florio, P., additional, Petraglia, F., additional, Bruce, K. D., additional, Sadek, K. H., additional, Macklon, N., additional, Cagampang, F. R., additional, Cheong, Y., additional, Goudakou, M., additional, Kalogeraki, A., additional, Matalliotakis, I., additional, Papatheodorou, A., additional, Pasadaki, T., additional, Karkanaki, A., additional, Prapas, I., additional, Panagiotidis, I., additional, Kasapi, E., additional, Barlow, D., additional, Oliver, J., additional, Loumaye, E., additional, Khanmohammadi, M., additional, kazemnejad, S., additional, darzi, S., additional, Khanjani, S., additional, Zarnani, A., additional, Akhondi, M., additional, Tan, C. W., additional, Ng, C. P., additional, Loh, S. F., additional, Tan, H. H., additional, Choolani, M., additional, Griffith, L., additional, Chan, J., additional, Andersson, K. L., additional, Sundqvist, J., additional, Scarselli, G., additional, Gemzell-Danielsson, K., additional, Lalitkumar, P. G., additional, Jana, S., additional, Chattopadhyay, R., additional, Datta Ray, C., additional, Chaudhury, K., additional, Chakravarty, B. N., additional, Hannan, N., additional, Evans, J., additional, Hincks, C., additional, Rombauts, L. J. F., additional, Salamonsen, L. A., additional, Choi, D., additional, Lee, J., additional, Park, J., additional, Chang, H., additional, Kim, M., additional, Hwang, K., additional, Takeuchi, K., additional, Kurematsu, T., additional, Fukumoto, Y., additional, Yuki, Y., additional, Kuroki, Y., additional, Homan, Y., additional, Sata, Y., additional, Takeuchi, M., additional, Munoz Munoz, E., additional, Ortiz Olivera, G., additional, Fernandez Lopez, I., additional, Martinez Martinez, B., additional, Aguilar Prieto, J., additional, Portela Perez, S., additional, Pellicer Martinez, A., additional, Keltz, M., additional, Sauerbrun, M., additional, Breborowicz, A., additional, Gonzales, E., additional, Vicente-Munoz, S., additional, Puchades-Carrasco, L., additional, Morcillo, I., additional, Hidalgo, J. J., additional, Gilabert-Estelles, J., additional, Novella-Maestre, E., additional, Pellicer, A., additional, Pineda-Lucena, A., additional, Yavorovskaya, K. A., additional, Okhtyrskaya, T. A., additional, Demura, T. A., additional, Faizulina, N. M., additional, Ezhova, L. S., additional, Kogan, E. A., additional, Bilibio, J. P., additional, Souza, C. A. B., additional, Rodini, G. P., additional, Genro, V., additional, Andreoli, C. G., additional, de Conto, E., additional, Cunha-Filho, J. S. L., additional, Saare, M., additional, Soritsa, D., additional, Jarva, L., additional, Vaidla, K., additional, Palta, P., additional, Laan, M., additional, Karro, H., additional, Soritsa, A., additional, Salumets, A., additional, Peters, M., additional, Miskova, A., additional, Pilmane, M., additional, Rezeberga, D., additional, Assou, S., additional, Letur, H., additional, Piomboni, P., additional, Stendardi, A., additional, Gambera, L., additional, De Leo, V., additional, Focarelli, R., additional, Tamm, K., additional, Simm, J., additional, Metsis, M., additional, Vodolazkaia, A., additional, Fassbender, A., additional, Kyama, C. M., additional, Bokor, A., additional, Schols, D., additional, Huskens, D., additional, Meuleman, C., additional, Peeraer, K., additional, Tomassetti, C., additional, D'Hooghe, T. M., additional, Machens, K., additional, Afhuppe, W., additional, Schulz, A., additional, Diefenbach, K., additional, Schutt, B., additional, Faustmann, T., additional, Reischl, J., additional, Altmae, S., additional, Reimand, J., additional, Laisk, T., additional, Hovatta, O., additional, Kolde, R., additional, Vilo, J., additional, Stavreus-Evers, A., additional, Lee, J. H., additional, Kim, S. G., additional, Kim, Y. Y., additional, Park, I. H., additional, Sun, H. G., additional, Lee, K. H., additional, Ezoe, K., additional, Kawano, H., additional, Yabuuchi, A., additional, Ochiai, K., additional, Nagashima, H., additional, Osada, H., additional, Kagawa, N., additional, Kato, O., additional, Tamura, I., additional, Asada, H., additional, Taketani, T., additional, Tamura, H., additional, Sugino, N., additional, Garcia Velasco, J., additional, Prieto, L., additional, Quesada, J. F., additional, Cambero, O., additional, Toribio, M., additional, Hur, C. Y., additional, Lim, K. S., additional, Lee, W. D., additional, Lim, J. H., additional, Germeyer, A., additional, Nelson, L., additional, Graham, A., additional, Jauckus, J., additional, Strowitzki, T., additional, Lessey, B., additional, Gyulmamedova, I., additional, Illina, O., additional, Illin, I., additional, Mogilevkina, I., additional, Chaika, A., additional, Nosenko, O., additional, Boykova, I., additional, Gulmamedova, E., additional, Isik, H., additional, Moraloglu, O., additional, Seven, A. L. I., additional, Kilic, S., additional, Erkayiran, U., additional, Caydere, M., additional, Batioglu, S., additional, Alhalabi, M., additional, Samawi, S., additional, Taha, A., additional, Kafri, N., additional, Modi, S., additional, Khatib, A., additional, Sharif, J., additional, Othman, A., additional, Lancuba, S., additional, Branzini, C., additional, Lopez, M., additional, Baricalla, A., additional, Cristina, C., additional, Chen, J., additional, Jiang, Y., additional, Zhen, X., additional, Hu, Y., additional, Yan, G., additional, Sun, H., additional, Mizumoto, J., additional, Ueno, J., additional, Carvalho, F. M., additional, Casals, G., additional, Ordi, J., additional, Guimera, M., additional, Creus, M., additional, Fabregues, F., additional, Casamitjana, R., additional, Carmona, F., additional, Balasch, J., additional, Choi, Y. S., additional, Kim, K. C., additional, Kim, K. H., additional, Lee, B. S., additional, Kim, S. H., additional, Overbergh, L., additional, Verdrengh, E., additional, Kyama, C., additional, Waelkens, E., additional, Mathieu, C., additional, Iwasa, T., additional, Hatano, K., additional, Hasegawa, E., additional, Ito, H., additional, Isaka, K., additional, L. Rocha, A. L., additional, Reis, F., additional, Lee, K. S., additional, Joo, J. K., additional, Son, J. B., additional, Choi, J. R., additional, Vidali, A., additional, Barad, D. H., additional, Gleicher, N., additional, Sayyah-Melli, M., additional, and Kazemi-Shishvan, M., additional

Published
2011
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17. Session 45: PCOS1

Author

Tso, L. O., primary, Costello, M. F., additional, Andriolo, R. B., additional, Albuquerque, L. E., additional, Freitas, V., additional, Morin - Papunen, L., additional, Rantala, A., additional, Unkila-Kallio, L., additional, Tiitinen, A., additional, Hippelainen, M., additional, Tinkanen, H., additional, Perheentupa, A., additional, Ruokonen, A., additional, Tapanainen, J. S., additional, Tang, T., additional, Barth, J. H., additional, Balen, A. H., additional, Lee, K., additional, Choi, Y. S., additional, Yang, H., additional, Seo, S. K., additional, Kim, H. Y., additional, Lee, B. S., additional, Germeyer, A., additional, Jauckus, J., additional, Zorn, M., additional, Toth, B., additional, Capp, E., additional, and Strowitzki, T., additional

Published
2010
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18. Posters * Fertility Preservation

Author

Talevi, R., primary, Barbato, V., additional, Mollo, V., additional, De Stefano, C., additional, Finelli, F., additional, Ferraro, R., additional, Gualtieri, R., additional, Zhou, P., additional, Liu, A. H., additional, Cao, Y. X., additional, Roman, H., additional, Pura, I., additional, Tarta, O., additional, Bourdel, N., additional, Marpeau, L., additional, Sabourin, J. C., additional, Portmann, M., additional, Nagy, Z. P., additional, Behr, B., additional, Alvaro Mercadal, B., additional, Demeestere, I., additional, Imbert, R., additional, Englert, Y., additional, Delbaere, A., additional, Lueke, S., additional, Buendgen, N., additional, Koester, F., additional, Diedrich, K., additional, Griesinger, G., additional, Kim, A., additional, Han, J. E., additional, Eunmi, C., additional, Kim, Y. S., additional, Cho, J. H., additional, Yoon, T. K., additional, Piomboni, P., additional, Stendardi, A., additional, Palumberi, D., additional, Morgante, G., additional, De Leo, V., additional, Serafini, F., additional, Focarelli, R., additional, Tatone, C., additional, Di Emidio, G., additional, Carbone, M. C., additional, Vento, M., additional, Ciriminna, R., additional, Artini, P. G., additional, Kyono, K., additional, Ishikawa, T., additional, Usui, K., additional, Hatori, M., additional, Yasmin, L., additional, Sato, E., additional, Iwasaka, M., additional, Fujii, K., additional, Owada, N., additional, Sankai, T., additional, McLaughlin, M., additional, Fineron, P., additional, Anderson, R. A., additional, Wallace, W. H. B., additional, Telfer, E. E., additional, Labied, S., additional, Beliard, A., additional, Munaut, C., additional, Foidart, J. M., additional, Turkcuoglu, I., additional, Oktay, K., additional, Rodriguez-Wallberg, K., additional, Kuwayama, M., additional, Takayama, Y., additional, Mori, C., additional, Kagawa, N., additional, Akakubo, N., additional, Takehara, Y., additional, Kato, K., additional, Leibo, S. P., additional, Kato, O., additional, Yoon, H., additional, Shin, Y., additional, cha, J., additional, Kim, H., additional, Lee, W., additional, Yoon, S., additional, Lim, J., additional, Larman, M. G., additional, Gardner, D. K., additional, Zander-Fox, D., additional, Lane, M., additional, Hamilton, H., additional, Lee, S., additional, Ozkavukcu, S., additional, Heytens, E., additional, Alappat, R. M., additional, Sole, M., additional, Boada, M., additional, Biadiu, M., additional, Santalo, J., additional, Coroleu, B., additional, Barri, P. N., additional, Veiga, A., additional, Rossi, L., additional, Bartoletti, R., additional, Mengarelli, M., additional, Boccia Artieri, G., additional, Gemini, L., additional, Mazzoli, L., additional, Giannini, L., additional, Scaravelli, G., additional, Silber, S. J., additional, Yamanguchi, S., additional, Nagumo, Y., additional, Takai, Y., additional, Ishihara, S., additional, Soleimani, R., additional, Rottiers, I., additional, Gojayev, A., additional, Cuvelier, A. C., additional, De Sutter, P., additional, Salama, M., additional, Winkler, K., additional, Murach, K. F., additional, Hofer, S., additional, Wildt, L., additional, Friess, S. C., additional, Okumura, N., additional, Kuji, N., additional, Kishimi, A., additional, Nishio, H., additional, Mochimaru, Y., additional, Minegishi, K., additional, Miyakoshi, K., additional, Fujii, T., additional, Tanaka, M., additional, Aoki, D., additional, Yoshimura, Y., additional, Hasegawa, K., additional, Juanzi, S., additional, Zhao, W., additional, Zhang, S., additional, Xue, X., additional, Silber, S., additional, Zhang, J., additional, Meirow, D., additional, Gosden, R., additional, Westphal, J. R., additional, Gerritse, R., additional, Beerendonk, C. C. M., additional, Braat, D. D. M., additional, Peek, R., additional, Coticchio, G., additional, Dal Canto, M., additional, Brambillasca, F., additional, Mignini Renzini, M., additional, Merola, M., additional, Lain, M., additional, Fadini, R., additional, Nottola, S. A., additional, Albani, E., additional, Lorenzo, C., additional, Carlini, T., additional, Maione, M., additional, Borini, A., additional, Macchiarelli, G., additional, Levi-Setti, P. E., additional, Rienzi, L., additional, Romano, S., additional, Capalbo, A., additional, Iussig, B., additional, Albricci, L., additional, Colamaria, S., additional, Baroni, E., additional, Sapienza, F., additional, Giuliani, M., additional, Anniballo, R., additional, Ubaldi, F. M., additional, Beyer, D. A., additional, Schultze-Mosgau, A., additional, Amari, F., additional, Al-Hasani, S., additional, Resta, S., additional, Magli, M. C., additional, Ruberti, A., additional, Lappi, M., additional, Ferraretti, A. P., additional, Gianaroli, L., additional, Prisant, N., additional, Belloc, S., additional, Cohen-Bacrie, M., additional, Hazout, A., additional, Olivennes, F., additional, Aubriot, F. X., additional, Alvarez, S., additional, De Mouzon, J., additional, Thieulin, C., additional, Cohen-Bacrie, P., additional, Wozniak, S., additional, Szkodziak, P., additional, Wozniakowska, E., additional, Paszkowski, M., additional, Paszkowski, T., additional, Diaz, D., additional, Dragnic, S., additional, Hayward, B., additional, Bennett, R., additional, Al-Sabbagh, A., additional, Novella-Maestre, E., additional, Teruel, J., additional, Carmona, L., additional, Rosello, E., additional, Pellicer, A., additional, Sanchez-Serrano, M., additional, Lee, J. R., additional, Lee, J. Y., additional, Kim, C. H., additional, Lee, Y., additional, Jee, B. C., additional, Suh, C. S., additional, Kim, S. H., additional, Moon, S. Y., additional, Mirabet, V., additional, Crespo, J., additional, Schiewe, M., additional, Nugent, N., additional, Zozula, S., additional, Anderson, R., additional, Zulategui, J. F., additional, Meseguer, M., additional, Remohi, J., additional, Castello, D., additional, Romero, J. L. L., additional, De los Santos, M. J., additional, Cobo, A. C., additional, von Wolff, M., additional, Jauckus, J., additional, Kupka, M., additional, Strowitzki, T., additional, Lawrenz, B., additional, Raanani, H., additional, Kaufman, B., additional, Maman, E., additional, Mendel, M. M., additional, Dor, J., additional, Buendgen, N. K., additional, Combelles, C., additional, Wang, H. Y., additional, Racowsky, C., additional, Kuleshova, L., additional, Tucker, M., additional, Graham, J., additional, Richter, K., additional, Carter, J., additional, and Levy, M., additional

Published
2010
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23. Intrauterine instillation of diluted seminal plasma at oocyte pick-up does not increase the IVF pregnancy rate: a double-blind, placebo controlled, randomized study

Author

von Wolff, M., Rösner, S., Germeyer, A., Jauckus, J., Griesinger, G., Strowitzki, T., von Wolff, M., Rösner, S., Germeyer, A., Jauckus, J., Griesinger, G., and Strowitzki, T.

Abstract

STUDY QUESTION Does intrauterine application of diluted seminal plasma (SP) at the time of ovum pick-up improve the pregnancy rate by ≥14% in IVF treatment? SUMMARY ANSWER Intrauterine instillation of diluted SP at the time of ovum pick-up is unlikely to increase the pregnancy rate by ≥14% in IVF. WHAT IS KNOWN ALREADY SP modulates endometrial function, and sexual intercourse around the time of embryo transfer has been suggested to increase the likelihood of pregnancy. A previous randomized double-blind pilot study demonstrated a strong trend towards increased pregnancy rates following the intracervical application of undiluted SP. As this study was not conclusive and as the finding could have been confounded by sexual intercourse, the intrauterine application of diluted SP was investigated in the present trial. STUDY DESIGN, SIZE, DURATION A single-centre, prospective, double-blind, placebo-controlled, randomized, superiority trial on women undergoing IVF was conducted from April 2007 until February 2012 at the University Department of Gynaecological Endocrinology and Reproductive Medicine, Heidelberg, Germany. PARTICIPANTS/MATERIALS, SETTING, METHODS The study was powered to detect an 14% increase in the clinical pregnancy rate and two sequential tests were planned using the Pocock spending function. At the first interim analysis, 279 women had been randomly assigned to intrauterine diluted SP (20% SP in saline from the patients' partner) (n = 138) or placebo (n = 141) at the time of ovum pick-up. MAIN RESULTS AND THE ROLE OF CHANCE The clinical pregnancy rate per randomized patient was 37/138 (26.8%) in the SP group and 41/141 (29.1%) in the placebo group (difference: −2.3%, 95% confidence interval of the difference: −12.7 to +8.2%; P = 0.69). The live birth rate per randomized patient was 28/138 (20.3%) in the SP group and 33/141 (23.4%) in the placebo group (difference: −3.1%, 95% confidence interval of the difference: −12.7 to +6.6%; P = 0.56). It was decided

24. Changes in the expression of cancer- and metastasis-related genes and proteins after metformin treatment under different metabolic conditions in endometrial cancer cells.

Author

Lange C, Brüggemann J, Thüner T, Jauckus J, Strowitzki T, and Germeyer A

Abstract

Research Question: Hyperinsulinemia and elevated estrogen levels are known risk factors for endometrial cancer (EC) development and are associated with obesity, type 2 diabetes mellitus (T2DM), insulin resistance, among others. Metformin, an insulin-sensitizing drug, displays anti-tumor effects in cancer patients, including EC, but the mechanism of action is still not completely understood. In the present study, the effects of metformin on gene and protein expression were investigated in pre- and postmenopausal EC in vitro models in order to identify candidates that are potentially involved in the drug's anti-cancer mechanism., Design: After treating the cells with metformin (0.1 and 1.0 mmol/L), changes in the expression of >160 cancer- and metastasis-related gene transcripts were evaluated with RNA arrays. A total of 19 genes and 7 proteins were selected for a follow-up expression analysis, including further treatment conditions, in order to evaluate the influence of hyperinsulinemia and hyperglycemia on metformin-induced effects., Results: Changes in the expression of BCL2L11, CDH1, CDKN1A, COL1A1, PTEN, MMP9 and TIMP2 were analyzed on gene and protein level. The consequences resulting from the detected expression changes as well as the influence of varying environmental influences are discussed in detail. With the presented data, we contribute to a better understanding of the direct anti-cancer activity of metformin as well as its underlying mechanism of action in EC cells., Conclusions: Although further research will be necessary to confirm the data, the influence of different environmental settings on metformin-induced effects could be highlighted with the presented data. Additionally, gene and protein regulation were not similar in the pre- and postmenopausal in vitro models., Competing Interests: The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (© 2023 The Authors.)

Published
2023
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25. Glucose and fatty acids catabolism during in vitro decidualization of human endometrial stromal cells.

Author

Citrinovitz ACM, Hauke J, Jauckus J, Langhans CD, Schwarz K, Zorn M, Strowitzki T, Okun JG, and Germeyer A

Subjects
Female, Humans, Metabolic Networks and Pathways, Fatty Acids metabolism, Stromal Cells, Cells, Cultured, Glucose metabolism, Endometrium metabolism
Abstract

The differentiation of endometrial stromal cells, named decidualization, is essential for the proper formation of the materno-fetal interphase. One important feature of decidualization is the increased glucose consumption and its utilization by endometrial cells to produce energy. Besides glucose, fatty acids are another important energy source for living cells and it has been described that endometrial stromal cells rely on the proper function of the oxidation of fatty acids for the correct decidualization. It is, however, unknown whether the turn-over of fatty acid degradation is modified during decidualization. Furthermore, it is also unknown how the final products of glucose and fatty acid catabolism are related to the function of the tricarboxylic acid cycle for the efficient ATP production. In this study, we evaluated the content levels of different intermediate metabolites and the expression of the key enzymes related to the degradation of glucose and fatty acids during the in vitro decidualization of human endometrial stromal cells. Our results suggest that human endometrial stromal cells undergo energetic metabolic changes during decidualization and that decidualizing and non-decidualizing cells differ in the level of activation of different metabolic pathways and, probably, in the use of intermediate metabolites., (© 2022. The Author(s).)

Published
2022
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26. GRN, NOTCH3, FN1, and PINK1 expression in eutopic endometrium - potential biomarkers in the detection of endometriosis - a pilot study.

Author

Holzer I, Machado Weber A, Marshall A, Freis A, Jauckus J, Strowitzki T, and Germeyer A

Subjects
Biomarkers metabolism, Endometriosis pathology, Endometrium metabolism, Endometrium pathology, Female, Gene Expression Regulation genetics, Humans, Pilot Projects, Endometriosis genetics, Fibronectins genetics, Progranulins genetics, Protein Kinases genetics, Receptor, Notch3 genetics
Abstract

Purpose: Endometriosis (EM) is a common gynecological disease affecting 10-15% of women of reproductive age. However, molecular mechanisms and pathogenesis are still not completely understood. Furthermore, due to the absence of a reliable clinical biomarker, the only viable method for the often-delayed definitive diagnosis is laparoscopic surgery. Our objective was to analyze molecular differences of selected endometrial proteins and genes of women suffering from different stages of EM compared with healthy women to evaluate potential clinical biomarkers., Methods: We analyzed eutopic endometrial tissue samples from women undergoing a laparoscopic surgery (n = 58). mRNA gene expression of progranulin (GRN), neurogenic locus notch homolog protein (NOTCH3), fibronectin (FN1), and PTEN-induced kinase 1 (PINK1) was analyzed using qRT-PCR. Protein expression was determined using ELISA and immunohistochemistry., Results: Significant differences in gene expression between the different stages of the disease were noted for GRN, NOTCH3, FN1, and PINK1 (p < 0.05). The endometrium of women with minimal EM (ASRM I) showed the highest mRNA expression. Protein levels of GRN and FN1 on the other hand were significantly decreased in the endometrium of women with EM compared with those of healthy controls. Furthermore, for GRN and FN1, we could detect a correlation of protein expression with the severity of the disease., Conclusion: Our findings suggest a potential use of GRN and FN1 as clinical biomarkers to detect endometriosis. In addition, GRN, NOTCH3, FN1, and PINK1 could potentially be useful to differentiate between the underlying stages of the disease. However, a validation with a larger study population is needed.

Published
2020
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27. In vitro maturation of immature oocytes from ovarian tissue prior to shipment to a cryobank.

Author

Dietrich JE, Jauckus J, Hoffmann S, Liebenthron J, Capp E, Strowitzki T, and Germeyer A

Subjects
Adult, Female, Humans, Prospective Studies, Young Adult, Cryopreservation methods, Fertility Preservation methods, In Vitro Oocyte Maturation Techniques methods, Oocyte Retrieval methods, Oocytes physiology
Abstract

Purpose: Female fertility preservation prior to gonadotoxic therapies can be achieved by the cryopreservation of ovarian cortical tissue. Immature oocytes may be recovered during the preparation, matured in vitro and lead to live births, thereby providing an additional option for fertility preservation. The purpose of this study was to test the feasibility of this approach in a setting with unilateral biopsy of a small piece of ovarian tissue and minimal tissue preparation prior to shipment to an external cryobank., Methods: A prospective observational clinical study in an academic center was performed from January 2018 through December 2019. Ovarian tissue was obtained laparoscopically. Immature oocytes were recovered by minimal preparation of the tissue before shipment to an external cryobank for cryopreservation. In vitro maturation was performed on recovered immature oocytes., Results: Twelve patients were enrolled. Immature oocytes could be recovered for all. The maturation rate was 38.9% (n = 14/36). Metaphase II (MII) were either directly used for intracytoplasmic sperm injection (ICSI) with a fertilization rate of 66.6% (n = 4/6) or vitrified (n = 8). PNs were cryopreserved (n = 4). Vitrified MII were warmed with a post-warming vitality rate of 75.0% (n = 3/4) and used for ICSI with a fertilization rate of 33.3% (n = 1/3)., Conclusions: Immature oocytes can be successfully retrieved from ovarian tissue through minimal tissue preparation prior to shipment to a cryobank, matured in vitro, fertilized and cryopreserved for potential future fertility treatments. The total number of oocytes available for fertility preservation can be increased even without controlled ovarian stimulation in a situation where only ovarian biopsy for cryopreservation is performed., Trial Registration: German Clinical Trials Register (DRKS), DRKS00013170. Registered 11 December 2017, https://www.drks.de/drks&#95;web/navigate.do?navigationId=trial.HTML&TRIAL&#95;ID=DRKS00013170 .

Published
2020
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28. Endometrial expression of receptivity markers subject to ovulation induction agents.

Author

Freis A, Germeyer A, Jauckus J, Capp E, Strowitzki T, Zorn M, and Machado Weber A

Subjects
Adult, Biomarkers metabolism, Cells, Cultured, Chemokine CXCL12 genetics, Embryo Implantation drug effects, Female, Humans, Interleukin-8 genetics, Chorionic Gonadotropin pharmacology, Endometrium metabolism, Luteinizing Hormone pharmacology, Ovulation Induction methods
Abstract

Purpose: Implantation rates differ according to ovulation induction agents in ART. This study investigates the different local endometrial effects of LH- versus hCG-induced ovulation., Methods: Endometrial stromal cells from healthy patients were cultured with hCG or LH in different concentrations, supplemented with 250 ng/mL hCG and progesterone after 2 and 5 days. In addition after decidualization induction, cells were treated with hCG (50 or 250 ng/mL) or LH (10 or 50 ng/mL) for 3 days. Receptivity markers expression was evaluated by real-time quantitative PCR on day 3 and 6., Results: On day 3, non-decidualized cells treated with LH showed an increased expression of IGFBP1, IL-8 and CXCL12 compared to hCG. The expression pattern changed on day 6, where cells treated with hCG showed higher expression of implantation markers compared to LH-treated cells. Furthermore, on day 3, decidualized cells treated with hCG250 showed an increased IL8 and CXCL12 expression compared to LH10., Conclusions: LH seems to modulate the local endometrial expression of receptivity markers earlier compared to hCG; however, the effect is not sustained over time in cells without prior decidualization. Though, in decidualized cells, pattern changed and an earlier positive effect of hCG was shown on IL-8 and CXCL12.

Published
2019
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29. Cytokines in relation to hCG are significantly altered in asymptomatic women with miscarriage - a pilot study.

Author

Freis A, Schlegel J, Daniel V, Jauckus J, Strowitzki T, and Germeyer A

Subjects
Abortion, Spontaneous diagnosis, Adaptor Proteins, Signal Transducing blood, Adult, Female, Granulocyte Colony-Stimulating Factor blood, Humans, Interleukin 1 Receptor Antagonist Protein blood, Pilot Projects, Pregnancy, Pregnancy Trimester, First blood, Prognosis, Prospective Studies, Abortion, Spontaneous blood, Chemokines blood, Chorionic Gonadotropin blood, Cytokines blood
Abstract

Background: Spontaneous abortion is one of the most common complications in early pregnancy. A preventive test to identify women who will experience a miscarriage, even before first symptoms occur, is not established. Activation of maternal immunological tolerance seems to be essential for early fetal development and various cytokines have been described in different stages of pregnancy. Therefore, we aimed to investigate if chemokine levels at the time of pregnancy testing relative to human Choriogonadotropin (hCG) are altered in patients who will experience a miscarriage in this pregnancy., Methods: We obtained blood samples from 39 women. Dependent on the follow-up, patients with a positive pregnancy test were subsequently divided in two groups: ongoing pregnancy (n = 22) and miscarriage (n = 17) in this pregnancy. Immunological and endocrine profiling of maternal plasma at the time of pregnancy testing (5th week of gestation) was performed for each group at the time of pregnancy test using Multiplex and ELISA analysis., Results: hCG was significantly decreased in patients with abortion whereas levels of IL-1ra, MIP-1a and TNF-alpha were significantly increased. GCSF/ IL-1ra-ratio was 1.66-fold increased in patients with ongoing pregnancy. TGF-beta /MIP1a-ratio was significantly 3.45-times higher in patients with miscarriage. Comparing patients with ongoing pregnancy to patients experiencing a miscarriage, we could demonstrate significant alterations of the ratios MIP1a/hCG, IL-1ra/hCG, TNFalpha/hCG, MCP1/hCG, IL-6/hCG, TPO/hCG and TGF-beta1/hCG. The strongest effects were seen for the ratio MIP1a/hCG, IL-1ra/hCG and TNFalpha/hCG., Conclusions: We have shown that cytokines in relation to hCG after 4 weeks of gestation are significantly altered in women with miscarriage, promising potential as a prognostic biomarker.

Published
2018
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30. Expression of semaphorin class 3 is higher in the proliferative phase on the human endometrium.

Author

Ferreira GD, Capp E, Jauckus J, Strowitzki T, and Germeyer A

Subjects
Biopsy, Endometrium pathology, Enzyme-Linked Immunosorbent Assay, Female, Humans, Membrane Glycoproteins, Membrane Proteins, Nerve Tissue Proteins, Real-Time Polymerase Chain Reaction, Semaphorin-3A metabolism, Cell Proliferation genetics, Endometrium metabolism, Menstrual Cycle metabolism, Semaphorins genetics, Semaphorins metabolism
Abstract

Purpose: The semaphorins are related to angiogenesis and cell proliferation depending on the tissue. The purpose of this study was to assess gene expression of class 3 semaphorin (SEMA3A-F) and protein expression of semaphorin 3A (SEMA3A) within human endometrium throughout the menstrual cycle., Methods: Gene expression of SEMA3A-F was analyzed by real-time PCR (qRT-PCR) and protein expression of SEMA3A was analyzed by ELISA in endometrial biopsies in the proliferative and secretory phase of the menstrual cycle., Results: Gene expression of SEMA3A, SEMA3C, SEMA3D, and SEMA3E was statistically significant decreased in secretory compared to proliferative phase endometrium (p < 0.05). Accordingly, SEMA3A protein expression in the secretory phase was lower than protein expression in proliferative phase endometrium (p ≤ 0.05)., Conclusion: SEMA3A, 3C, 3D, and 3E are possibly related to cell proliferation in the endometrium, being more expressed in the proliferative phase of the cycle. This finding may stimulate studies of class 3 semaphorins as a possible target for treatment of endometrial pathologies.

Published
2018
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31. Altered miRNA-profile dependent on ART outcome in early pregnancy targets Wnt-pathway.

Author

Freis A, Keller A, Ludwig N, Meese E, Jauckus J, Rehnitz J, Capp E, Strowitzki T, and Germeyer A

Subjects
Adult, Embryo Culture Techniques, Embryo Implantation, Female, Fertility, Gene Expression Regulation, Developmental, Humans, Infertility genetics, Infertility metabolism, Infertility physiopathology, MicroRNAs genetics, Pilot Projects, Pregnancy, Pregnancy Rate, Prospective Studies, Sperm Injections, Intracytoplasmic, Time Factors, Transcriptome, Treatment Outcome, Wnt Proteins genetics, Wnt3 Protein genetics, Young Adult, Embryo Transfer adverse effects, Fertilization in Vitro adverse effects, Infertility therapy, MicroRNAs metabolism, Wnt Proteins metabolism, Wnt Signaling Pathway genetics, Wnt3 Protein metabolism
Abstract

Main goal of this study is to detect the possible alterations in microRNA (miRNA) expression and the pathway targeted in plasma at the time of embryo transfer and pregnancy testing dependent on the assisted reproductive treatment (ART) outcome after ovarian hyperstimulation for in vitro fertilization. Changes in miRNA expression in plasma of women, who became pregnant ( n  = 6) vs women who failed implantation ( n  = 6) following day 5 embryo transfer (ET), were investigated at the day of ET and pregnancy testing (PT). Protein expression to validate the finding was performed with a sample size of n  = 20 (10 per group) using enzyme-linked immunosorbent assay. Enriched Kyoto Encyclopedia of Genes and Genomes (KEGG) pathway analyses were performed using DIANA-miRPath, v3.0 software based on predicted targets by DIANA-microT-CDS. 4 miRNAs could be identified as possible biomarkers for implantation success. The 11 miRNAs showing the highest significant alterations were all associated with the regulation of WNT3 and WNT7a. While WNT7a presented with a significant decrease between ET and PT in case of ongoing pregnancy, women with implantation failure showed unaltered concentrations. WNT3 presented with a significant decrease in both groups. However, the loss of WNT3 between ET and PT was significantly higher in patients who became pregnant. Main limitation of this prospective study is its small sample size, defining it as a pilot analysis. To conclude, we could demonstrate a significant change in miRNA profile dependent on the ART outcome affecting Wnt pathway. Our findings indicate a possible prospective use of miRNA as biomarkers for implantation success., (© 2017 Society for Reproduction and Fertility.)

Published
2017
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32. Effects of a hyperandrogenaemic state on the proliferation and decidualization potential in human endometrial stromal cells.

Author

Freis A, Renke T, Kämmerer U, Jauckus J, Strowitzki T, and Germeyer A

Subjects
Adult, Decidua drug effects, Dexamethasone therapeutic use, Embryo Implantation drug effects, Endometrium cytology, Endometrium metabolism, Epithelial Cells cytology, Epithelial Cells metabolism, Female, Gene Expression Regulation drug effects, Humans, Insulin Resistance, Matrix Metalloproteinase 2 genetics, Matrix Metalloproteinase 2 metabolism, Metformin therapeutic use, Polycystic Ovary Syndrome drug therapy, Stromal Cells cytology, Stromal Cells metabolism, TOR Serine-Threonine Kinases genetics, TOR Serine-Threonine Kinases metabolism, Testosterone, Cell Proliferation drug effects, Dexamethasone adverse effects, Endometrium drug effects, Epithelial Cells drug effects, Metformin adverse effects, Stromal Cells drug effects
Abstract

Objective: Polycystic ovary syndrome (PCOS) is the most common endocrine disorder in women, involving hyperandrogenaemia and insulin resistance. Treatment options include dexamethasone, as well as the off-label use of metformin. To evaluate the impact of those drugs on cyclic changes in endometrial development, we tested possible effects of metformin and dexamethasone on endometrial stromal cells decidualisation, proliferation, and gene regulation in a hyperandrogenaemic microenvironment in vitro., Methods/design: Ten endometrial biopsies (of which five were decidualized in vitro) were used from regularly cycling women. Cells were treated with testosterone, dexamethasone, and metformin in different concentrations. Thereafter, cells were assessed for proliferation and decidualization capacity, as well as mTor and MMP-2 gene regulation., Results: Metformin showed a dose-dependent negative effect on prolactin secretion, a known decidualization marker. This effect was stronger in a hyperandrogenaemic condition and could not be compensated by dexamethasone. Testosterone had a dose dependent negative effect on proliferation in decidualized endometrial stromal cells. Dexamethasone slightly compensated the negative proliferative effect only in low-dose testosterone. High-dose metformin also showed a dose-dependent reduction in endometrial stromal cell proliferation without a major impact by testosterone or dexamethasone in decidualized and non-decidualized cells. High-dose metformin significantly reduced the expression of matrix metalloproteinase-2 (MMP-2) and mechanistic Target of Rapamycin (mTor), regardless of the concentration of dexamethasone and testosterone. The strongest effect could be observed for the combination with high-dose dexamethasone., Conclusion: When therapies, such as metformin and dexamethasone, are used to normalize peripheral androgen levels in patients with PCOS, their effect on the endometrial microenvironment should be taken into consideration as well, especially metformin has to be used with caution because of its dose dependent, possibly inhibiting effect at the endometrial proliferation.

Published
2017
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33. Proliferation and metastatic potential of endometrial cancer cells in response to metformin treatment in a high versus normal glucose environment.

Author

de Barros Machado A, Dos Reis V, Weber S, Jauckus J, Brum IS, von Eye Corleta H, Strowitzki T, Capp E, and Germeyer A

Abstract

In order to improve our understanding of the potential preventive and therapeutic role of metformin, the present study aimed to investigate the capability of low-dose metformin in the efficient inhibition of cancer development and the reduction of the metastasis of endometrial adenocarcinoma type I and primary endometrial epithelial cells (eEPs), with the drug acting as a treatment in a hyperinsulinemic environment exposed to high and normal glucose conditions. The Ishikawa endometrial adenocarcinoma cell line and primary eEPs were exposed to an environment with high (17 mM) or normal glucose (5 mM) and treated with insulin, low-dose metformin (0.1 mM) or a combined treatment. Metastatic potential was assessed by migration and invasion assays, and relative cell proliferation was determined. Metformin at a low dose potently inhibited the insulin action, decreasing the ability of the endometrial cancer (EC) cell line to migrate and invade in a high and normal glucose environment, and decreasing the migration ability of the primary eEPs. In the EC cell line, the insulin treatment increased the proliferation, without any subsequent reduction of proliferation by the addition of 0.1 mM metformin; however, relative cell proliferation sensitivity to metformin was observed in the range between 1 and 5 mM regardless of the glucose concentration present. Overall, metformin at 0.1 mM is not efficient enough to decrease the proliferation in an EC cell line. However, at this concentration, metformin can inhibit the insulin action in endometrial epithelial cancer cells, demonstrating an anti-metastatic effect in high and normal glucose environments.

Published
2016
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34. Timing of ovarian stimulation in patients prior to gonadotoxic therapy: an analysis of 684 stimulations.

Author

von Wolff M, Capp E, Jauckus J, Strowitzki T, and Germeyer A

Subjects
Adult, Female, Fertilization in Vitro, Humans, Incidence, Oocyte Retrieval, Ovarian Hyperstimulation Syndrome epidemiology, Ovulation Induction adverse effects, Pregnancy, Registries, Retrospective Studies, Time Factors, Fertility Preservation methods, Ovarian Hyperstimulation Syndrome etiology, Ovulation Induction methods
Abstract

Objective: Time to therapy initiation in patients requiring gonadotoxic therapy is crucial. This article evaluates the efficiency of random start ovarian stimulation in affected women., Study Design: Retrospective anonymous registry data analysis from 85 university and non-university fertility centres participating in the international network FertiPROTEKT. The study comprised 684 women undergoing ovarian stimulation for fertility preservation from 2007 to 2013. According to the time of stimulation initiation, days of ovarian stimulation, total dose of gonadotropins used, gonadotropin dose used per day, number of oocytes retrieved and incidence of ovarian hyperstimulation syndrome were analysed. Statistical analysis was performed using analysis of variance in case of continuous outcome variables and chi-square tests in case of categorical variables., Results: Among 684 women who underwent ovarian stimulation prior to gonadotoxic therapy 472 (69.0%) started ovarian stimulation between menstrual cycle day 1-5 (group A), 109 (15.9%) between day 6-14 (group B) and 103 (15.1%) after day 14 (group C). The days of stimulation (A: 10.8±2.4, B: 10.6±2.7, C: 11.5±2.2) and total dose of gonadotropins (A: 2496IU±980, B: 2529IU±940, C: 2970IU±1145) were significantly increased in group C. Numbers of obtained oocytes (Group A: 11.6±7.7, B: 13.9±9.1, C: 13.6±7.9) were significantly increased in group B and C, while the overall incidence of ovarian hyperstimulation syndrome III° was 0.15%., Conclusion: The outcome of ovarian stimulation is similar after stimulation initiation during any phase of the menstrual cycles, supporting the concept of random-start ovarian stimulation before gonadotoxic therapy without disadvantage for the patient concerning later fertility preservation., (Copyright © 2016 Elsevier Ireland Ltd. All rights reserved.)

Published
2016
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35. Modulation of the IGF system and proliferation in human endometrial stromal cells by metformin: a dose-dependent effect.

Author

Jung ML, Renke T, Nowak O, Jauckus J, Zorn M, Capp E, Strowitzki T, and Germeyer A

Subjects
Cells, Cultured, Dose-Response Relationship, Drug, Endometrium drug effects, Epithelial Cells metabolism, Female, Humans, Hypoglycemic Agents administration & dosage, Insulin-Like Growth Factor Binding Protein 1 genetics, Insulin-Like Growth Factor Binding Protein 1 metabolism, Insulin-Like Growth Factor I genetics, Insulin-Like Growth Factor I metabolism, Insulin-Like Growth Factor II genetics, Insulin-Like Growth Factor II metabolism, Metformin administration & dosage, Progesterone pharmacology, Prolactin genetics, Prolactin metabolism, Receptor, IGF Type 1 genetics, Receptor, IGF Type 1 metabolism, Stromal Cells drug effects, Embryo Implantation drug effects, Endometrium metabolism, Hypoglycemic Agents pharmacology, Metformin pharmacology, Stromal Cells metabolism
Abstract

Purpose: To assess the metformin effect on endometrial stromal cell decidualization, proliferation, gene and protein expression of IGFBPs, IGFs and their receptors., Methods: Human endometrial stromal cells (hESCs) were cultured from endometrial biopsies of 11 women undergoing surgery for benign reasons. hESCs were decidualized with and without metformin in increasing doses. Supernatant and cells were harvested after decidualization for 12-14 days, followed by real-time PCR of IGFBP 1-6, IGF I, IGF II and their receptors. Prolactin, and IGFBP-1, -3, and -6 were additionally analyzed in supernatant by ELISA. Proliferation of hESCs and decidualization of hESCs were assessed under the influence of metformin. Data were analyzed using the paired t test with p < 0.05 considered significant., Results: While lower concentrations of metformin (10(-4), 10(-5 )M) did not influence the decidualization and proliferation capacity of hESCs, higher concentrations (10(-3), 10(-2 )M metformin) significantly (p < 0.05) diminished decidualization, as well as stromal cell proliferation in a dose-dependent manner. Higher concentrations of metformin lead to a significant (p < 0.05) dose-dependent attenuation of the progesterone effect with regard to IGFBP-1, -3, -5, -6, as well as IGF I receptor, while it did not change the expression of IGFBP-2 and -4, IGF I and II and the IGF II receptor. This was confirmed on the protein level for IGFBP-1, -3, and -6., Conclusion: We were able to demonstrate for the first time a dose-dependent local effect of metformin within hESCs. Metformin might therefore influence locally the endometrial proliferation and maturation, and could open up new treatment options for gynecological diseases by vaginal application of metformin.

Published
2015
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36. Endometrial beta3 integrin profile reflects endometrial receptivity defects in women with unexplained recurrent pregnancy loss.

Author

Germeyer A, Savaris RF, Jauckus J, and Lessey B

Subjects
Adult, Biomarkers metabolism, Biopsy, Case-Control Studies, Down-Regulation, Endometrium pathology, Endometrium physiopathology, Female, Fertility, Germany, Humans, Immunohistochemistry, Luteinizing Hormone urine, North Carolina, Retrospective Studies, Uterine Diseases pathology, Uterine Diseases physiopathology, Uterine Diseases urine, Abortion, Habitual etiology, Embryo Implantation, Endometrium metabolism, Integrin beta3 metabolism, Luteal Phase, Uterine Diseases metabolism
Abstract

Background: The pathophysiology of recurrent pregnancy loss (RPL) is still unknown in 50% of the cases. Herein we measure the expression of beta3 integrin subunit, a well-known implantation marker, in women with or without RPL and correlate it with the histological dating of the endometrial tissue., Methods: LH-timed endometrial biopsies were obtained from cases (RPL; n = 21, age 33.9+/-4.7) and healthy controls (n = 29; age 29.8+/-4.1) during the mid-secretory phase (post ovulatory day: 8 to 10). Endometrial samples were timed histologically according to Noyes' criteria and underwent immunohistochemical staining for beta3 integrin expression. For statistical analysis the semi-quantitative HSCORE was assessed. Type I (beta3 negative in an out-of-phase endometrium) and Type II defect (beta3 negative in an in-phase endometrium) were also analysed. Statistical analysis was done with Student t-test, Mann Whitney U test, ANCOVA and chi square for trend. Significance was set as P < 0.05., Results: The mean (SD) age in controls was lower compared to cases [(29.8 (4.1) vs. 33.9 (4.7) - P = 0.001; Student t-test)]. The median (range) expression of beta3 integrin in controls and cases was 1.94 (0 to 3.5) vs. 0.82 (0 to 3.6), respectively (P = 0.001; Mann Whitney U test). Significance was still significant after adjusting for age (P = 0.03;ANCOVA). The normal positive staining > =0.7 of beta3 integrin subunit and in-phase endometrium was seen in 24 out of 29 (82.8%) controls, but in only 6 out of 21 (28.6%) of cases with RPL; Type I and II defects were seen in 10.3 and 6.9% of controls, while present in 52.4 and 19.1% of cases, respectively (P = 0.0005; chi-square)., Conclusions: Women with unexplained RPL had significantly reduced integrin expression compared to controls. Our findings underline the need for further molecular analysis of endometrial tissue in affected women.

Published
2014
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37. Modulation of tumor necrosis factor-stimulated gene-6 (TSG-6) expression in human endometrium.

Author

Capp E, Milner CM, Williams J, Hauck L, Jauckus J, Strowitzki T, and Germeyer A

Subjects
Abortion, Habitual metabolism, Biopsy, Case-Control Studies, Cell Adhesion Molecules genetics, Cells, Cultured, Endometrium pathology, Enzyme-Linked Immunosorbent Assay, Female, Fluorescent Antibody Technique, Follicular Phase metabolism, Humans, Luteal Phase metabolism, Placenta metabolism, Pregnancy, Real-Time Polymerase Chain Reaction, Up-Regulation, Cell Adhesion Molecules metabolism, Endometrium metabolism, RNA, Messenger metabolism, Stromal Cells metabolism
Abstract

Introduction: The human endometrium undergoes repetitive, cyclical changes under the influence of endocrine signals (estrogen and progesterone). In particular, the extensive tissue remodeling, angiogenesis and leukocyte infiltration that occur during decidualization of the endometrium give rise to an environment that is permissive to blastocyst attachment. However, it is now well established that crosstalk (via paracrine signals) between the trophoblast and the endometrium is also a key for successful implantation. Microarray studies have identified TSG-6 as a gene with elevated expression in endometrial stromal cells following the exposure to trophoblast and immune cell products. TSG-6 is an inflammation-associated protein which acts as a potent inhibitor of neutrophil extravasation and also plays important roles in matrix remodeling, e.g., by promoting hyaluronan (HA) cross-linking and down-regulating the protease network. Female TSG-6 (-/-) mice are infertile and this has been attributed to their inability to ovulate; however, the importance of TSG-6 in implantation has not been directly investigated., Material and Methods: Real-time PCR, as well as immunofluorescence staining was performed on endometrial biopsies of proliferative and secretory phase samples. In addition stromal cell cultures of human endometrium were used to assess the influence of different stimulating factors on the TSG-6 gene and protein expression via real-time PCR and ELISA., Results: Herein demonstrate that TSG-6 mRNA is expressed by the endometrium during the proliferative and secretory phases of the menstrual cycle. We also show that conditioned media from placental tissues induce rapid upregulation of TSG-6 mRNA expression and sustained protein secretion, with evidence that TNF is an important factor in this effect. Furthermore, we demonstrate changes in protein expression in the mid-secretory phase in women affected by recurrent abortions., Conclusion: These data suggest that TSG-6 expression might be essential in endometrial matrix organization and feto-maternal communication during the implantation process.

Published
2014
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38. Cell-type specific expression and regulation of apolipoprotein D and E in human endometrium.

Author

Germeyer A, Capp E, Schlicksupp F, Jauckus J, von Rango U, von Wolff M, and Strowitzki T

Subjects
Apolipoproteins D biosynthesis, Apolipoproteins D metabolism, Apolipoproteins E biosynthesis, Apolipoproteins E metabolism, Cells, Cultured, Female, Humans, RNA, Messenger biosynthesis, Up-Regulation genetics, Apolipoproteins D genetics, Apolipoproteins E genetics, Endometrium cytology, Endometrium metabolism, Gene Expression Regulation
Abstract

Objective: To assess the expression and regulation of antilipoprotein D (ApoD) and antilipoprotein E (ApoE) in human endometrium., Study Design: Endometrial biopsies from healthy, regularly cycling women were collected during the late proliferative and mid-secretory phase. mRNA gene expression of ApoD and ApoE was determined using real-time PCR in whole tissue, in isolated stromal (ESC), epithelial (EEC) and CD45(+) leukocytes (EIC), as well as after hormonal stimulation of ESC and EEC in vitro. Protein expression was analyzed using immunohistochemistry., Results: ApoD and ApoE mRNA was expressed in all cell types examined. A rise in ApoD mRNA expression was seen in whole endometrium, ESC, and EEC in the secretory phase, as well as after hormonal stimulation of ESC and EEC in vitro. ApoE mRNA was significantly upregulated in whole endometrium of secretory phase biopsies, while its expression was not altered by progesterone in vitro. Immunohistochemistry of whole endometrial tissue localized ApoD mainly in ESC and EEC. While ApoE was localized slightly in ESC, it was particularly noted on the surface of secretory phase endothelial cells., Conclusion: We demonstrate for the first time the cell-type and cycle dependent expression of ApoD and ApoE within human endometrium, suggesting their role in endometrial modulation., (Copyright © 2013 Elsevier Ireland Ltd. All rights reserved.)

Published
2013
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39. Does metformin influence the insulin-, IGF I- and IGF II-receptor gene expression and Akt phosphorylation in human decidualized endometrial stromal cells?

Author

Capp E, Jauckus J, von Eye Corleta H, Toth B, Strowitzki T, and Germeyer A

Subjects
Cells, Cultured, Female, Gene Expression drug effects, Humans, Insulin pharmacology, Insulin-Like Growth Factor I pharmacology, Insulin-Like Growth Factor II pharmacology, Phosphorylation, Proto-Oncogene Proteins c-akt metabolism, Stromal Cells drug effects, Endometrium drug effects, Insulin genetics, Metformin pharmacology, Receptor, IGF Type 1 genetics, Receptor, IGF Type 2 genetics, Reproductive Control Agents pharmacology
Abstract

Objective: To assess the effects of metformin on insulin-, IGF I-, and IGF II-receptor gene expression and Akt phosphorylation in decidualized human endometrial stromal cells (ESC) after stimulation with insulin, IGF I and II., Study Design: ESC were isolated from healthy, regularly cycling women and after two passages decidualized with estrogen/progesterone±metformin. Cells were incubated with insulin, IGF I or IGF II for 1, 5, and 10 min to assess Akt phosphorylation by Western blot. To investigate the insulin-, IGF I- and IGF II-receptor gene expression ESC were incubated with insulin, IGF I or IGF II for 6 and 24h., Results: Insulin- and IGF I-receptor gene expression in ESC changed significantly after incubation with insulin, IGF I or IGF II. This was further augmented in metformin pretreated cells, while IGF II-receptor gene expression changed particularly after pretreatment with metformin. Akt phosphorylation peaked after 5 min insulin, IGF I and IGF II stimulation in ESC in both control (control 0.08 ± 0.03 vs. insulin 0.74 ± 0.19, IGF I 0.68 ± 0.22, IGF II 0.53 ± 0.13, p<0.05) and metformin pretreated cells (control 0.03 ± 0.01 vs. insulin 0.75 ± 0.11, IGF I 0.74 ± 0.15, IGF II 0.67 ± 0.09, p<0.005). However, there was no significant difference between the control and metformin pretreated group., Conclusion: Insulin, IGF I and IGF II lead to changes in their receptor gene expression and induced Akt phosphorylation in ESC. These effects were further highlighted in the presence of metformin., (Copyright © 2011 Elsevier Ireland Ltd. All rights reserved.)

Published
2011
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40. Metformin modulates IL-8, IL-1β, ICAM and IGFBP-1 expression in human endometrial stromal cells.

Author

Germeyer A, Jauckus J, Zorn M, Toth B, Capp E, and Strowitzki T

Subjects
Endometrium metabolism, Enzyme-Linked Immunosorbent Assay, Female, Gonadal Steroid Hormones, Humans, In Vitro Techniques, Insulin, Prolactin metabolism, Stromal Cells metabolism, Endometrium cytology, Gene Expression Regulation drug effects, Insulin-Like Growth Factor Binding Protein 1 metabolism, Intercellular Adhesion Molecule-1 metabolism, Interleukin-1beta metabolism, Interleukin-8 metabolism, Metformin pharmacology
Abstract

To evaluate the effects of metformin on endometrial stromal cell gene expression and on the decidualization process, endometrial biopsies were collected from five healthy, regularly cycling women. Stromal cell culture was performed and decidualized with oestrogen/progesterone in the presence or absence of metformin and thereafter stimulated with insulin. The effect of metformin on decidualization was analysed by prolactin determination in the cell culture supernatant. Gene expression of insulin-like growth factor binding protein 1 (IGFBP-1), interleukin (IL) 8 and 1β and intercellular adhesion molecule (ICAM) was analysed by real-time PCR. Decidualization was significantly diminished in cells incubated with metformin (P<0.05) accompanied by a significant reduction of prolactin secretion in the supernatant (day 10: 2.2 fold, P<0.05; day 15: 3.1 fold, P<0.05). IGFBP-1 gene expression was reduced after long-term metformin exposure (7.7 fold, P<0.05). The negative effect of insulin on IL-8 (4.8 fold) and IL-1β (9.3 fold) gene expression was similarly found in cells incubated with metformin. As far as is known, this is the first demonstration of a change in endometrial gene and protein expression after in-vitro stimulation with metformin, including a diminished decidualization process and changes in genes relevant to implantation., (Copyright © 2010 Reproductive Healthcare Ltd. Published by Elsevier Ltd. All rights reserved.)

Published
2011
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41. Fertility preservation in >1,000 patients: patient's characteristics, spectrum, efficacy and risks of applied preservation techniques.

Author

Lawrenz B, Jauckus J, Kupka MS, Strowitzki T, and von Wolff M

Subjects
Adolescent, Adult, Austria, Breast Neoplasms drug therapy, Cryopreservation, Female, Germany, Gonadotropin-Releasing Hormone adverse effects, Gonadotropin-Releasing Hormone agonists, Hodgkin Disease drug therapy, Humans, Ovulation Induction adverse effects, Registries, Switzerland, Tissue Preservation, Young Adult, Antineoplastic Agents adverse effects, Infertility, Female prevention & control, Reproductive Techniques, Assisted adverse effects
Abstract

Introduction: Data on the characteristics of female patients counselled for fertility preservation and the efficacy and risk of the applied procedures are still poor. We therefore analysed the registry of a network of 70 infertility centers which are involved in fertility preservation in Germany, Switzerland and Austria, called FertiPROTEKT ( hhtp://www.fertiprotekt.eu )., Materials and Methods: 1,280 counselled patients (15-40 years) were analysed regarding characteristics and different fertility preservation treatments before cytotoxic therapy in 2007-2009., Results: 34.8% of the counselled patients were diagnosed with breast cancer, 30.5% with Hodgkin's lymphoma, 25.4% with other malignancies and 9.3% with non-malignant diseases. 89.6% of the treated breast cancer patients were 25-40 years of age, and 87.5% of the lymphoma patients were 15-30 years of age. At the time of counselling, 85.3% of the breast cancer patients and 92.7% of the lymphoma patients were childless. 1,080 patients received a single or combined therapy such as GnRH agonists (n = 823), cryopreservation of ovarian tissue (n = 500), ovarian stimulation (n = 221) and transposition of the ovaries (n = 24). Only one severe complication, requiring postponement of the chemotherapy, was documented. In stimulated patients, 2,417 oocytes (mean n = 11.6, SD ± 7.7) were received. Fertilisation rate per received oocyte was 61.3%., Conclusions: Fertility preservation programmes mainly involve women without children, diagnosed with breast cancer or Hodgkin's lymphoma. Fertility preservation techniques can be applied with low risk. The limited and age-dependant success rate of the different therapies require individualised approaches of single or combined fertility preservation techniques.

Published
2011
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42. Efficacy and safety of ovarian stimulation before chemotherapy in 205 cases.

Author

Lawrenz B, Jauckus J, Kupka M, Strowitzki T, and von Wolff M

Subjects
Adolescent, Adult, Antineoplastic Combined Chemotherapy Protocols adverse effects, Cryopreservation methods, Drug Administration Schedule, Female, Follow-Up Studies, Humans, Infertility, Female etiology, Neoplasms complications, Oocytes, Pregnancy, Pregnancy Rate, Registries, Time Factors, Treatment Outcome, Young Adult, Antineoplastic Combined Chemotherapy Protocols administration & dosage, Infertility, Female prevention & control, Neoplasms drug therapy, Ovulation Induction adverse effects, Ovulation Induction methods
Abstract

Ovarian stimulation and cryopreservation of fertilized oocytes before cancer therapy is the best established and efficient fertility preservation technique and should still be considered before chemotherapy. Within a short time frame of 2 weeks, between 8.6 (18-25 y) and 5.1 (36-40 y) fertilized oocytes can be cryopreserved., (Copyright © 2010 American Society for Reproductive Medicine. Published by Elsevier Inc. All rights reserved.)

Published
2010
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43. Changes in cell proliferation, but not in vascularisation are characteristic for human endometrium in different reproductive failures--a pilot study.

Author

Germeyer A, von Wolff M, Jauckus J, Strowitzki T, Sharma T, and Grazul-Bilska AT

Subjects
Abortion, Spontaneous etiology, Abortion, Spontaneous metabolism, Adult, Case-Control Studies, Endometrium metabolism, Female, Humans, Ki-67 Antigen metabolism, Pilot Projects, Pregnancy, Abortion, Spontaneous pathology, Cell Proliferation, Endometrium blood supply, Endometrium pathology, Neovascularization, Physiologic physiology
Abstract

Background: Reproductive failure, determined as recurrent spontaneous abortions (RSA) or recurrent implantation failure (RIF) in women is not well understood. Several factors, including embryo quality, and cellular and molecular changes in endometrium may contribute to the insufficient feto-maternal interaction resulting in reproductive failure. Prior clinical studies suggest an inadequate endometrial growth and development of the endometrium, leading to a lesser endometrial thickness., Methods: We therefore aimed to determine the cellular proliferation using Ki67, and the expression of markers of vascularisation, such as factor VIII (a marker of endothelial cells) and smooth muscle cell actin (SMCA; a marker of pericytes and smooth muscle cells) in endometrium of healthy women and women with RSA or RIF. LH-dated mid-secretory endometrial biopsies of seven healthy women and twenty women with reproductive failure were examined via immunohistochemistry followed by image analysis., Results: Cellular proliferation but not expression of factor VIII or SMCA was decreased (P < 0.0004) in endometrium of women with RSA and RIF compared to healthy controls., Conclusion: Our data indicate that reproductive failure is due to insufficient cell proliferation/tissue growth rather than inadequate vascularisation in the endometrium.

Published
2010
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44. Intravaginal and intracervical application of seminal plasma in in vitro fertilization or intracytoplasmic sperm injection treatment cycles--a double-blind, placebo-controlled, randomized pilot study.

Author

von Wolff M, Rösner S, Thöne C, Pinheiro RM, Jauckus J, Bruckner T, Biolchi V, Alia A, and Strowitzki T

Subjects
Adult, Cervix Uteri physiology, Double-Blind Method, Female, Humans, Infertility etiology, Insemination, Artificial methods, Male, Patient Selection, Pilot Projects, Placebos, Pregnancy, Pregnancy Outcome, Pregnancy Rate, Treatment Failure, Vagina physiology, Young Adult, Fertilization in Vitro methods, Semen physiology, Sperm Injections, Intracytoplasmic methods, Spermatozoa physiology
Abstract

Objective: To evaluate whether intravaginal application of seminal plasma at the time of follicle aspiration in IVF or intracytoplasmic sperm injection treatment cycles has the potential to increase pregnancy rate. To calculate the number of patients needed to achieve significance in a multicenter trial., Design: Double-blind, placebo-controlled randomized pilot study., Setting: University department of gynecological endocrinology and reproductive medicine., Patient(s): One hundred sixty-eight patients undergoing IVF or intracytoplasmic sperm injection treatment., Intervention(s): Cryopreserved seminal plasma from the patient's partner or sodium chloride (placebo) was injected into the cervix and the posterior fornix of the vagina just after follicle aspiration., Main Outcome Measure(s): Clinical-pregnancy rate., Result(s): One hundred sixty-eight patients agreed to participate in the study. Participation was limited to one treatment cycle. Thirty-one patients (18%) were excluded from the study, mainly as a result of canceled embryo transfers. Seventy patients received placebo, and 67 received seminal plasma. The clinical-pregnancy rate was 25.7% (18/70) in the placebo group. The clinical-pregnancy rate in the seminal plasma group reached 37.3% (25/67), corresponding to a relative increase of 45%., Conclusion(s): Even though significance was not reached in this pilot study, the data suggest that seminal plasma has the potential to improve pregnancy rate. It is estimated that around 450 patients need to be recruited to reach significance in a multicenter study.

Published
2009
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45. The long pentraxin PTX3 in human endometrium: regulation by steroids and trophoblast products.

Author

Popovici RM, Krause MS, Jauckus J, Germeyer A, Brum IS, Garlanda C, Strowitzki T, and von Wolff M

Subjects
Adult, Biopsy, C-Reactive Protein genetics, Cells, Cultured, Embryo Implantation physiology, Endometrium drug effects, Endometrium pathology, Female, Humans, Menstrual Cycle metabolism, RNA, Messenger metabolism, Serum Amyloid P-Component genetics, Stromal Cells metabolism, Stromal Cells pathology, C-Reactive Protein metabolism, Endometrium metabolism, Estrogens physiology, Interleukin-1beta physiology, Progesterone physiology, Serum Amyloid P-Component metabolism, Trophoblasts physiology
Abstract

Human implantation is characterized by blastocyst attachment to endometrial epithelial cells followed by invasion of trophoblast into the maternal decidua. There has been an increasing amount of data linking higher levels of the pentraxin PTX3, a long pentraxin, to embryo implantation. PTX3 levels were found to be higher in patients with preeclampsia and intrauterine growth restriction, both conditions caused by faulty implantation. Furthermore, PTX3 knockout mice have reduced fertility due to cumulus oopherus malformation as well as implantation failure. In a human implantation model, we and others have shown that trophoblast action on endometrial stromal cells induces PTX3 expression. In this study, we analyzed PTX3 expression throughout the menstrual cycle as well as its regulation by hormones involved in the implantation process. We also compared PTX3 expression in stromal cells induced by trophoblast conditioned medium to its induction by trophoblast coculture. PTX3 mRNA expression in human endometrial stromal cells is regulated by progesterone, estrogen, and IL-1 but not human chorionic gonadotropin and is increased by both trophoblast-conditioned medium as well as trophoblast explants. PTX3 protein production and regulation by these factors is shown by Western blot. Based on these findings, we conclude that estradiol and progesterone are involved in PTX3 induction and regulation during implantation. Also, of the factors secreted by trophoblast, IL-1beta induces PTX3 in human endometrial stromal cells.

Published
2008
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46. Gene expression profiling of human endometrial-trophoblast interaction in a coculture model.

Author

Popovici RM, Betzler NK, Krause MS, Luo M, Jauckus J, Germeyer A, Bloethner S, Schlotterer A, Kumar R, Strowitzki T, and von Wolff M

Subjects
Adult, Cell Culture Techniques, Embryo Implantation, Endometrium metabolism, Female, Fluorescent Antibody Technique methods, Gene Expression, Humans, Models, Biological, Pregnancy, Trophoblasts metabolism, Coculture Techniques methods, Endometrium cytology, Gene Expression Profiling methods, Trophoblasts cytology
Abstract

Investigating the interaction of human endometrium and trophoblast during implantation is difficult in vitro and impossible in vivo. This study was designed to analyze the effect of trophoblast on endometrial stromal cells during implantation by comprehensive gene profiling. An in vitro coculture system of endometrial stromal cells with first-trimester trophoblast explants was established. Trophoblast and endometrial stromal cells were separated after 24 h. Gene expression of endometrial stromal cells after coculture was compared with the gene expression of endometrial stromal cells cultured alone by microarray analysis. We confirmed the expression of distinct genes using real-time PCR. Genes up-regulated included those for inflammatory response, immune response, and chemotaxis (pentraxin-related gene 3, chemokine ligands, IL-8, IL-1 receptors, IL-18 receptor, IL-15, IL-15 receptor, TNF-alpha-induced protein 6, and IL-6 signal transducer), regulators of cell growth (IGF-binding proteins 1 and 2) and signal transduction. Also up-regulated were genes for growth and development, glucose metabolism, and lipid metabolism: DKK-1, WISP, IGF-II, hydroxysteroid 11beta-dehydrogenase 1, hydroxyprostaglandin dehydrogenase 15, prostaglandin E synthase, prostaglandin F receptor, aldehyde dehydrogenase 1 family, member A3 and phosphatidic acid phosphatase type 2B. Other genes included genes for cell-cell signaling (pre-B-cell colony-enhancing factor 1), proteolysis, calcium ion binding, regulation of transcription, and others. Down-regulated genes included genes for proteolysis (MMP-11 and mitochondrial intermediate peptidase), genes for cell death (caspase 6, death-associated protein kinase 1, and histone deacetylase 5), transcription factors (sex determining region Y-box 4, dachshund homolog 1, ets variant gene 1, and zinc finger protein 84 and 435), and genes for humoral immune response (CD24 antigen). Trophoblast has a significant impact on endometrial stromal cell gene expression. Some of the genes regulated by trophoblast in endometrial stromal cells are already known to be regulated by progesterone and show the endocrine function of trophoblast during pregnancy. Others are genes so far unknown to play a role in endometrial-trophoblast interaction and open a wide field of investigation.

Published
2006
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47. Regulation of matrix metalloproteinases and their inhibitors in uterine endometrial cells of patients with and without endometriosis.

Author

Sillem M, Prifti S, Koch A, Neher M, Jauckus J, and Runnebaum B

Subjects
Adult, Cells, Cultured, Diethylstilbestrol pharmacology, Female, Humans, Interleukin-1 pharmacology, Matrix Metalloproteinase 1 metabolism, Matrix Metalloproteinase 2 metabolism, Matrix Metalloproteinase 3 metabolism, Matrix Metalloproteinase 9 metabolism, Promegestone pharmacology, Tissue Inhibitor of Metalloproteinase-1 metabolism, Tissue Inhibitor of Metalloproteinase-2 metabolism, Tumor Necrosis Factor-alpha pharmacology, Endometriosis enzymology, Endometrium enzymology, Matrix Metalloproteinases metabolism, Tissue Inhibitor of Metalloproteinases metabolism
Abstract

Objective: To determine whether alterations in the secretion and regulation of matrix metalloproteinases (MMPs) and their inhibitors are present in uterine endometrial cells from endometriosis patients., Study Design: In an in vitro study, uterine endometrial cells from 19 regularly cycling women with and 32 without endometriosis were treated with diethyl stilbestrol, promegestone (R5020), interleukin-1 (IL-1) and tumor necrosis factor a (TNF-alpha). Culture supernatants were assayed for MMPs 1, 2, 3, and 9, and for tissue inhibitors of MMP (TIMP-1 and TIMP-2) by ELISA., Results: MMP-3 was secreted in high concentrations, moderate concentrations were seen for MMP-1 and MMP-2, and very low concentrations for MMP-9. Substantially more TIMP-1 than TIMP-2 was secreted. MMP-1 and MMP-3 were uniformly attenuated by R5020, while MMP-2 was not influenced by hormone treatment. MMP-3 was upregulated by TNF-alpha in all samples while IL-1 only increased secretion in cells from endometriosis patients., Conclusion: The upregulation of MMP-3 by IL-1 may contribute to an increased invasiveness of uterine endometrial fragments in endometriosis patients.

Published
2001
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