Your search keyword '"Młynarz P"' showing total 39 results

1. Serum metabolite and metal ions profiles for breast cancer screening

Author

Wojtowicz, Wojciech, Tarkowski, R., Olczak, A., Szymczycha-Madeja, A., Pohl, P., Maciejczyk, A., Trembecki, Ł., Matkowski, R., and Młynarz, Piotr

Published

2024

2. A single dose of glycogen phosphorylase inhibitor improves cognitive functions of aged mice and affects the concentrations of metabolites in the brain

Author

Pudełko-Malik, Natalia, Drulis-Fajdasz, Dominika, Pruss, Łukasz, Mielko-Niziałek, Karolina Anna, Rakus, Dariusz, Gizak, Agnieszka, and Młynarz, Piotr

Published

2024

3. Author Correction: Examination of internal metabolome and VOCs profile of brewery yeast and their mutants producing beer with improved aroma

Author

Jabłoński, Sławomir Jan, Mielko-Niziałek, Karolina Anna, Leszczyński, Przemysław, Gasiński, Alan, Kawa-Rygielska, Joanna, Młynarz, Piotr, and Łukaszewicz, Marcin

Published

2024

4. Examination of internal metabolome and VOCs profile of brewery yeast and their mutants producing beer with improved aroma

Author

Jabłoński, Sławomir Jan, Mielko-Niziałek, Karolina Anna, Leszczyński, Przemysław, Gasiński, Alan, Kawa-Rygielska, Joanna, Młynarz, Piotr, and Łukaszewicz, Marcin

Published

2024

5. The oxidative stress and metabolic response of Acinetobacter baumannii for aPDT multiple photosensitization

Author

Wanarska, Ewelina, Mielko, Karolina Anna, Maliszewska, Irena, and Młynarz, Piotr

Published

2022

6. Phytochemicals containing biologically active polyphenols as an effective agent against Covid-19-inducing coronavirus

Author

Chojnacka, K., Witek-Krowiak, A., Skrzypczak, D., Mikula, K., and Młynarz, P.

Published

2020

7. Brain-dead and coma patients exhibit different serum metabolic profiles: preliminary investigation of a novel diagnostic approach in neurocritical care

Author

Dawiskiba, Tomasz, Wojtowicz, Wojciech, Qasem, Badr, Łukaszewski, Marceli, Mielko, Karolina Anna, Dawiskiba, Agnieszka, Banasik, Mirosław, Skóra, Jan Paweł, Janczak, Dariusz, and Młynarz, Piotr

Published

2021

8. Comparison of bacteria disintegration methods and their influence on data analysis in metabolomics

Author

Mielko, Karolina Anna, Jabłoński, Sławomir Jan, Łukaszewicz, Marcin, and Młynarz, Piotr

Published

2021

9. Inclusive J/psi production in pp collisions at sqrt(s) = 2.76 TeV

Author

ALICE Collaboration, Abelev, B., Adam, J., Adamova, D., Adare, A. M., Aggarwal, M. M., Rinella, G. Aglieri, Agocs, A. G., Agostinelli, A., Salazar, S. Aguilar, Ahammed, Z., Masoodi, A. Ahmad, Ahmad, N., Ahn, S. U., Akindinov, A., Aleksandrov, D., Alessandro, B., Molina, R. Alfaro, Alici, A., Alkin, A., Avina, E. Almaraz, Alme, J., Alt, T., Altini, V., Altinpinar, S., Altsybeev, I., Andrei, C., Andronic, A., Anguelov, V., Anielski, J., Anson, C., Anticic, T., Antinori, F., Antonioli, P., Aphecetche, L., Appelshauser, H., Arbor, N., Arcelli, S., Arend, A., Armesto, N., Arnaldi, R., Aronsson, T., Arsene, I. C., Arslandok, M., Asryan, A., Augustinus, A., Averbeck, R., Awes, T. C., Aysto, J., Azmi, M. D., Bach, M., Badala, A., Baek, Y. W., Bailhache, R., Bala, R., Ferroli, R. Baldini, Baldisseri, A., Baldit, A., Pedrosa, F. Baltasar Dos Santos, Ban, J., Baral, R. C., Barbera, R., Barile, F., Barnafoldi, G. G., Barnby, L. S., Barret, V., Bartke, J., Basile, M., Bastid, N., Bathen, B., Batigne, G., Batyunya, B., Baumann, C., Bearden, I. G., Beck, H., Belikov, I., Bellini, F., Bellwied, R., Belmont-Moreno, E., Bencedi, G., Beole, S., Berceanu, I., Bercuci, A., Berdnikov, Y., Berenyi, D., Bergmann, C., Berzano, D., Betev, L., Bhasin, A., Bhati, A. K., Bianchi, L., Bianchi, N., Bianchin, C., Bielcik, J., Bielcikova, J., Bjelogrlic, S., Blanco, F., Blau, D., Blume, C., Boccioli, M., Bock, N., Bogdanov, A., Boggild, H., Bogolyubsky, M., Boldizsar, L., Bombara, M., Book, J., Borel, H., Borissov, A., Bose, S., Bossu, F., Botje, M., Bottger, S., Boyer, B., Braidot, E., Braun-Munzinger, P., Bregant, M., Breitner, T., Browning, T. A., Broz, M., Brun, R., Bruna, E., Bruno, G. E., Budnikov, D., Buesching, H., Bufalino, S., Bugaiev, K., Busch, O., Buthelezi, Z., Orduna, D. Caballero, Caffarri, D., Cai, X., Caines, H., Villar, E. Calvo, Camerini, P., Roman, V. Canoa, Romeo, G. Cara, Carena, W., Carena, F., Filho, N. Carlin, Carminati, F., Montoya, C. A. Carrillo, Diaz, A. Casanova, Castellanos, J. Castillo, Hernandez, J. F. Castillo, Casula, E. A. R., Catanescu, V., Cavicchioli, C., Cepila, J., Cerello, P., Chang, B., Chapeland, S., Charvet, J. L., Chattopadhyay, S., Chawla, I., Cherney, M., Cheshkov, C., Cheynis, B., Chiavassa, E., Barroso, V. Chibante, Chinellato, D. D., Chochula, P., Chojnacki, M., Christakoglou, P., Christensen, C. H., Christiansen, P., Chujo, T., Chung, S. U., Cicalo, C., Cifarelli, L., Cindolo, F., Cleymans, J., Coccetti, F., Colamaria, F., Colella, D., Balbastre, G. Conesa, del Valle, Z. Conesa, Constantin, P., Contin, G., Contreras, J. G., Cormier, T. M., Morales, Y. Corrales, Cortese, P., Maldonado, I. Cortes, Cosentino, M. R., Costa, F., Cotallo, M. E., Crescio, E., Crochet, P., Alaniz, E. Cruz, Cuautle, E., Cunqueiro, L., Dainese, A., Dalsgaard, H. H., Danu, A., Das, K., Das, I., Das, D., Dash, A., Dash, S., De, S., de Barros, G. O. V., De Caro, A., de Cataldo, G., de Cuveland, J., De Falco, A., De Gruttola, D., Delagrange, H., Sanchez, E. Del Castillo, Deloff, A., Demanov, V., De Marco, N., Denes, E., De Pasquale, S., Deppman, A., Erasmo, G. D, de Rooij, R., Corchero, M. A. Diaz, Di Bari, D., Dietel, T., Di Giglio, C., Di Liberto, S., Di Mauro, A., Di Nezza, P., Divia, R., Djuvsland, O., Dobrin, A., Dobrowolski, T., Dominguez, I., Donigus, B., Dordic, O., Driga, O., Dubey, A. K., Ducroux, L., Dupieux, P., Majumdar, A. K. Dutta, Majumdar, M. R. Dutta, Elia, D., Emschermann, D., Engel, H., Erdal, H. A., Espagnon, B., Estienne, M., Esumi, S., Evans, D., Eyyubova, G., Fabris, D., Faivre, J., Falchieri, D., Fantoni, A., Fasel, M., Fearick, R., Fedunov, A., Fehlker, D., Feldkamp, L., Felea, D., Feofilov, G., Tellez, A. Fernandez, Ferreiro, E. G., Ferretti, A., Ferretti, R., Figiel, J., Figueredo, M. A. S., Filchagin, S., Finogeev, D., Fionda, F. M., Fiore, E. M., Floris, M., Foertsch, S., Foka, P., Fokin, S., Fragiacomo, E., Fragkiadakis, M., Frankenfeld, U., Fuchs, U., Furget, C., Girard, M. Fusco, Gaardhoje, J. J., Gagliardi, M., Gago, A., Gallio, M., Gangadharan, D. R., Ganoti, P., Garabatos, C., Garcia-Solis, E., Garishvili, I., Gerhard, J., Germain, M., Geuna, C., Gheata, A., Gheata, M., Ghidini, B., Ghosh, P., Gianotti, P., Girard, M. R., Giubellino, P., Gladysz-Dziadus, E., Glassel, P., Gomez, R., Gonzalez-Trueba, L. H., Gonzalez-Zamora, P., Gorbunov, S., Goswami, A., Gotovac, S., Grabski, V., Graczykowski, L. K., Grajcarek, R., Grelli, A., Grigoras, A., Grigoras, C., Grigoriev, V., Grigoryan, A., Grigoryan, S., Grinyov, B., Grion, N., Gros, P., Grosse-Oetringhaus, J. F., Grossiord, J. -Y., Grosso, R., Guber, F., Guernane, R., Gutierrez, C. Guerra, Guerzoni, B., Guilbaud, M., Gulbrandsen, K., Gunji, T., Gupta, A., Gupta, R., Gutbrod, H., Haaland, O., Hadjidakis, C., Haiduc, M., Hamagaki, H., Hamar, G., Han, B. H., Hanratty, L. D., Hansen, A., Harmanova, Z., Harris, J. W., Hartig, M., Hasegan, D., Hatzifotiadou, D., Hayrapetyan, A., Heckel, S. T., Heide, M., Helstrup, H., Herghelegiu, A., Corral, G. Herrera, Herrmann, N., Hetland, K. F., Hicks, B., Hille, P. T., Hippolyte, B., Horaguchi, T., Hori, Y., Hristov, P., Hrivnacova, I., Huang, M., Huber, S., Humanic, T. J., Hwang, D. S., Ichou, R., Ilkaev, R., Ilkiv, I., Inaba, M., Incani, E., Innocenti, G. M., Innocenti, P. G., Ippolitov, M., Irfan, M., Ivan, C., Ivanov, V., Ivanov, A., Ivanov, M., Ivanytskyi, O., Jacholkowski, A., Jacobs, P. M., Jancurova, L., Jang, H. J., Jangal, S., Janik, M. A., Janik, R., Jayarathna, P. H. S. Y., Jena, S., Bustamante, R. T. Jimenez, Jirden, L., Jones, P. G., Jung, H., Jusko, A., Kaidalov, A. B., Kakoyan, V., Kalcher, S., Kalinak, P., Kalisky, M., Kalliokoski, T., Kalweit, A., Kanaki, K., Kang, J. H., Kaplin, V., Uysal, A. Karasu, Karavichev, O., Karavicheva, T., Karpechev, E., Kazantsev, A., Kebschull, U., Keidel, R., Khan, M. M., Khan, S. A., Khan, P., Khanzadeev, A., Kharlov, Y., Kileng, B., Kim, M., Kim, J. S., Kim, D. J., Kim, T., Kim, B., Kim, S., Kim, S. H., Kim, D. W., Kim, J. H., Kirsch, S., Kisel, I., Kiselev, S., Kisiel, A., Klay, J. L., Klein, J., Klein-Bosing, C., Kliemant, M., Kluge, A., Knichel, M. L., Knospe, A. G., Koch, K., Kohler, M. K., Kolojvari, A., Kondratiev, V., Kondratyeva, N., Konevskikh, A., Korneev, A., Don, C. Kottachchi Kankanamge, Kour, R., Kowalski, M., Kox, S., Meethaleveedu, G. Koyithatta, Kral, J., Kralik, I., Kramer, F., Kraus, I., Krawutschke, T., Krelina, M., Kretz, M., Krivda, M., Krizek, F., Krus, M., Kryshen, E., Krzewicki, M., Kucheriaev, Y., Kuhn, C., Kuijer, P. G., Kurashvili, P., Kurepin, A., Kurepin, A. B., Kuryakin, A., Kushpil, S., Kushpil, V., Kvaerno, H., Kweon, M. J., Kwon, Y., de Guevara, P. Ladron, Lakomov, I., Langoy, R., Lara, C., Lardeux, A., La Rocca, P., Lazzeroni, C., Lea, R., Bornec, Y. Le, Lee, S. C., Lee, K. S., Lefevre, F., Lehnert, J., Leistam, L., Lenhardt, M., Lenti, V., Leon, H., Monzon, I. Leon, Vargas, H. Leon, Levai, P., Lien, J., Lietava, R., Lindal, S., Lindenstruth, V., Lippmann, C., Lisa, M. A., Liu, L., Loenne, P. I., Loggins, V. R., Loginov, V., Lohn, S., Lohner, D., Loizides, C., Loo, K. K., Lopez, X., Torres, E. Lopez, Lovhoiden, G., Lu, X. -G., Luettig, P., Lunardon, M., Luo, J., Luparello, G., Luquin, L., Luzzi, C., Ma, K., Ma, R., Madagodahettige-Don, D. M., Maevskaya, A., Mager, M., Mahapatra, D. P., Maire, A., Malaev, M., Cervantes, I. Maldonado, Malinina, L., Mal'Kevich, D., Malzacher, P., Mamonov, A., Manceau, L., Mangotra, L., Manko, V., Manso, F., Manzari, V., Mao, Y., Marchisone, M., Mares, J., Margagliotti, G. V., Margotti, A., Marin, A., Tobon, C. A. Marin, Markert, C., Martashvili, I., Martinengo, P., Martinez, M. I., Davalos, A. Martinez, Garcia, G. Martinez, Martynov, Y., Mas, A., Masciocchi, S., Masera, M., Masoni, A., Massacrier, L., Mastromarco, M., Mastroserio, A., Matthews, Z. L., Matyja, A., Mayani, D., Mayer, C., Mazer, J., Mazzoni, M. A., Meddi, F., Menchaca-Rocha, A., Perez, J. Mercado, Meres, M., Miake, Y., Milano, L., Milosevic, J., Mischke, A., Mishra, A. N., Miskowiec, D., Mitu, C., Mlynarz, J., Mohanty, A. K., Mohanty, B., Molnar, L., Zetina, L. Montano, Monteno, M., Montes, E., Moon, T., Morando, M., De Godoy, D. A. Moreira, Moretto, S., Morsch, A., Muccifora, V., Mudnic, E., Muhuri, S., Muller, H., Munhoz, M. G., Musa, L., Musso, A., Nandi, B. K., Nania, R., Nappi, E., Nattrass, C., Naumov, N. P., Navin, S., Nayak, T. K., Nazarenko, S., Nazarov, G., Nedosekin, A., Nicassio, M., Nielsen, B. S., Niida, T., Nikolaev, S., Nikolic, V., Nikulin, V., Nikulin, S., Nilsen, B. S., Nilsson, M. S., Noferini, F., Nomokonov, P., Nooren, G., Novitzky, N., Nyanin, A., Nyatha, A., Nygaard, C., Nystrand, J., Ochirov, A., Oeschler, H., Oh, S. K., Oh, S., Oleniacz, J., Oppedisano, C., Velasquez, A. Ortiz, Ortona, G., Oskarsson, A., Ostrowski, P., Otwinowski, J., Ovrebekk, G., Oyama, K., Ozawa, K., Pachmayer, Y., Pachr, M., Padilla, F., Pagano, P., Paic, G., Painke, F., Pajares, C., Pal, S. K., Pal, S., Palaha, A., Palmeri, A., Papikyan, V., Pappalardo, G. S., Park, W. J., Passfeld, A., Pastircak, B., Patalakha, D. I., Paticchio, V., Pavlinov, A., Pawlak, T., Peitzmann, T., Filho, E. Pereira De Oliveira, Peresunko, D., Lara, C. E. Perez, Lezama, E. Perez, Perini, D., Perrino, D., Peryt, W., Pesci, A., Peskov, V., Pestov, Y., Petracek, V., Petran, M., Petris, M., Petrov, P., Petrovici, M., Petta, C., Piano, S., Piccotti, A., Pikna, M., Pillot, P., Pinazza, O., Pinsky, L., Pitz, N., Piuz, F., Piyarathna, D. B., Ploskon, M., Pluta, J., Pocheptsov, T., Pochybova, S., Podesta-Lerma, P. L. M., Poghosyan, M. G., Polak, K., Polichtchouk, B., Pop, A., Porteboeuf-Houssais, S., Pospisil, V., Potukuchi, B., Prasad, S. K., Preghenella, R., Prino, F., Pruneau, C. A., Pshenichnov, I., Puchagin, S., Puddu, G., Teixido, J. Pujol, Pulvirenti, A., Punin, V., Putis, M., Putschke, J., Quercigh, E., Qvigstad, H., Rachevski, A., Rademakers, A., Radomski, S., Raiha, T. S., Rak, J., Rakotozafindrabe, A., Ramello, L., Reyes, A. Ramirez, Raniwala, S., Raniwala, R., Rasanen, S. S., Rascanu, B. T., Rathee, D., Read, K. F., Real, J. S., Redlich, K., Reichelt, P., Reicher, M., Renfordt, R., Reolon, A. R., Reshetin, A., Rettig, F., Revol, J. -P., Reygers, K., Riccati, L., Ricci, R. A., Richert, T., Richter, M., Riedler, P., Riegler, W., Riggi, F., Cahuantzi, M. Rodriguez, Roed, K., Rohr, D., Rohrich, D., Romita, R., Ronchetti, F., Rosnet, P., Rossegger, S., Rossi, A., Roukoutakis, F., Roy, C., Roy, P., Montero, A. J. Rubio, Rui, R., Ryabinkin, E., Rybicki, A., Sadovsky, S., Safarik, K., Sahoo, R., Sahu, P. K., Saini, J., Sakaguchi, H., Sakai, S., Sakata, D., Salgado, C. A., Salzwedel, J., Sambyal, S., Samsonov, V., Castro, X. Sanchez, Sandor, L., Sandoval, A., Sano, S., Sano, M., Santo, R., Santoro, R., Sarkamo, J., Scapparone, E., Scarlassara, F., Scharenberg, R. P., Schiaua, C., Schicker, R., Schmidt, H. R., Schmidt, C., Schreiner, S., Schuchmann, S., Schukraft, J., Schutz, Y., Schwarz, K., Schweda, K., Scioli, G., Scomparin, E., Scott, P. A., Scott, R., Segato, G., Selyuzhenkov, I., Senyukov, S., Seo, J., Serci, S., Serradilla, E., Sevcenco, A., Sgura, I., Shabetai, A., Shabratova, G., Shahoyan, R., Sharma, N., Sharma, S., Shigaki, K., Shimomura, M., Shtejer, K., Sibiriak, Y., Siciliano, M., Sicking, E., Siddhanta, S., Siemiarczuk, T., Silvermyr, D., Silvestre, C., Simonetti, G., Singaraju, R., Singh, R., Singha, S., Sinha, T., Sinha, B. C., Sitar, B., Sitta, M., Skaali, T. B., Skjerdal, K., Smakal, R., Smirnov, N., Snellings, R. J. M., Sogaard, C., Soltz, R., Son, H., Song, M., Song, J., Soos, C., Soramel, F., Sputowska, I., Spyropoulou-Stassinaki, M., Srivastava, B. K., Stachel, J., Stan, I., Stefanek, G., Stefanini, G., Steinbeck, T., Steinpreis, M., Stenlund, E., Steyn, G., Stocco, D., Stolpovskiy, M., Strabykin, K., Strmen, P., Suaide, A. A. P., Vasquez, M. A. Subieta, Sugitate, T., Suire, C., Sukhorukov, M., Sultanov, R., Sumbera, M., Susa, T., de Toledo, A. Szanto, Szarka, I., Szostak, A., Tagridis, C., Takahashi, J., Takaki, J. D. Tapia, Tauro, A., Munoz, G. Tejeda, Telesca, A., Terrevoli, C., Thader, J., Thomas, D., Tieulent, R., Timmins, A. R., Tlusty, D., Toia, A., Torii, H., Toscano, L., Tosello, F., Truesdale, D., Trzaska, W. H., Tsuji, T., Tumkin, A., Turrisi, R., Tveter, T. S., Ulery, J., Ullaland, K., Ulrich, J., Uras, A., Urban, J., Urciuoli, G. M., Usai, G. L., Vajzer, M., Vala, M., Palomo, L. Valencia, Vallero, S., van der Kolk, N., Vyvre, P. Vande, van Leeuwen, M., Vannucci, L., Vargas, A., Varma, R., Vasileiou, M., Vasiliev, A., Vechernin, V., Veldhoen, M., Venaruzzo, M., Vercellin, E., Vergara, S., Vernekohl, D. C., Vernet, R., Verweij, M., Vickovic, L., Viesti, G., Vikhlyantsev, O., Vilakazi, Z., Baillie, O. Villalobos, Vinogradov, A., Vinogradov, Y., Vinogradov, L., Virgili, T., Viyogi, Y. P., Vodopyanov, A., Voloshin, S., Voloshin, K., Volpe, G., von Haller, B., Vranic, D., Vrlakova, J., Vulpescu, B., Vyushin, A., Wagner, B., Wagner, V., Wan, R., Wang, Y., Wang, D., Wang, M., Watanabe, K., Wessels, J. P., Westerhoff, U., Wiechula, J., Wikne, J., Wilde, M., Wilk, G., Wilk, A., Williams, M. C. S., Windelband, B., Karampatsos, L. Xaplanteris, Yang, H., Yang, S., Yasnopolskiy, S., Yi, J., Yin, Z., Yokoyama, H., Yoo, I. -K., Yoon, J., Yu, W., Yuan, X., Yushmanov, I., Zach, C., Zampolli, C., Zaporozhets, S., Zarochentsev, A., Zavada, P., Zaviyalov, N., Zbroszczyk, H., Zelnicek, P., Zgura, I. S., Zhalov, M., Zhang, X., Zhou, D., Zhou, Y., Zhou, F., Zhu, X., Zichichi, A., Zimmermann, A., Zinovjev, G., Zoccarato, Y., and Zynovyev, M.

Subjects

High Energy Physics - Experiment

Abstract

The ALICE Collaboration has measured inclusive J/psi production in pp collisions at a center of mass energy sqrt(s)=2.76 TeV at the LHC. The results presented in this Letter refer to the rapidity ranges |y|<0.9 and 2.5

Published

2012

10. Serum metabolomics approach to monitor the changes in metabolite profiles following renal transplantation

Author

Stanimirova, Ivana, Banasik, Mirosław, Ząbek, Adam, Dawiskiba, Tomasz, Kościelska-Kasprzak, Katarzyna, Wojtowicz, Wojciech, Krajewska, Magdalena, Janczak, Dariusz, and Młynarz, Piotr

Published

2020

11. Metabolomic studies as a tool for determining the post-mortem interval (PMI) in stillborn calves

Author

Jawor, Paulina, Ząbek, Adam, Wojtowicz, Wojciech, Król, Dawid, Stefaniak, Tadeusz, and Młynarz, Piotr

Published

2019

12. Predisposition to atherosclerosis in children and adults with trisomy 21: biochemical and metabolomic studies.

Author

Hetman, Marta, Mielko, Karolina, Placzkowska, Sylwia, Bodetko, Aleksandra, Młynarz, Piotr, and Barg, Ewa

Subjects

DOWN syndrome, APOLIPOPROTEIN B, APOLIPOPROTEIN A, METABOLOMICS, LIPID metabolism, THREONINE, TYROSINE

Abstract

Introduction: Atherosclerosis, a precursor to cardiovascular disease (CVD), is deeply intertwined with lipid metabolism. The metabolic process in the Down syndrome (DS) population remain less explored. Aim of the study: This study examines the lipid profiles of DS in comparison to their siblings (CG), aiming to uncover potential atherosclerotic and CVD risks. Material and methods: The study included 42 people with DS (mean age 14.17 years) and the CG - 20 individuals (mean age 15.92 years). Anthropometric measurements: BMI, BMI SDS, and TMI were calculated. Lipid profile (LP) and metabolomics were determined. Results: LP: DS display significantly reduced HDL (DS vs. CG: 47±10 vs. 59 ±12 mg/dl; p = 0.0001) and elevated LDL (104 ±25 vs. 90 ±22 mg/dl; p = 0.0331). Triglycerides, APO A1, and APO B/APO A1 ratio corroborate with the elevated risk of CVD in DS. Despite no marked differences in: TCH and APO B, the DS group demonstrated a concerning BMI trend. Of 31 identified metabolites, 12 showed statistical significance (acetate, choline, creatinine, formate, glutamine, histidine, lysine, proline, pyroglutamate, threonine, tyrosine, and xanthine). However, only 8 metabolites passed the FDR validation (acetate, creatinine, formate, glutamine, lysine, proline, pyroglutamate, xanthine). Conclusions: Down syndrome individuals show distinct cardiovascular risks, with decreased HDL and increased LDL levels. Combined with metabolomic disparities and higher BMI and TMI, this suggests an increased atherosclerosis risk compared to controls. [ABSTRACT FROM AUTHOR]

Published

2023

13. Linear and Nonlinear Optical Properties of Azobenzene Derivatives Modified with an (Amino)naphthalene Moiety.

Author

Dudek, Marta, Kaczmarek-Kędziera, Anna, Deska, Radosław, Trojnar, Jakub, Jasik, Patryk, Młynarz, Piotr, Samoć, Marek, and Matczyszyn, Katarzyna

Published

2022

14. Metabolomics provides new information on the changes occurring in thyroid tumours

Author

Balcerzak, Waldemar, primary, Deja, S, additional, Młynarz, P, additional, Ząbek, A, additional, Orczyk-Pawiłowicz, M, additional, Głód, M, additional, Dawiskiba, T, additional, and Pawełka, D, additional

Published

2013

15. Bioelectrochemical synthesis of rhamnolipids and energy production and its correlation with nitrogen in air-cathode microbial fuel cells.

Author

de Rosset A, Tyszkiewicz N, Wiśniewski J, Pudełko-Malik N, Rutkowski P, Młynarz P, and Pasternak G

Subjects

Electrodes, Bioreactors, Bioelectric Energy Sources, Nitrogen metabolism, Surface-Active Agents metabolism, Glycolipids metabolism

Abstract

Microbial fuel cells (MFCs) have been recently proven to synthesise biosurfactants from waste products. In classic bioreactors, the efficiency of biosynthesis process can be controlled by the concentration of nitrogen content in the electrolyte. However, it was not known whether a similar control mechanism could be applied in current-generating conditions. In this work, the effect of nitrogen concentration on biosurfactant production from waste cooking oil was investigated. The concentration of NH 4 Cl in the electrolyte ranged from 0 to 1 g L -1 . The maximum power density equal to 17.5 W m -3 was achieved at a concentration of 0.5 g L -1 (C/N = 2.32) and was accompanied by the highest surface tension decrease (to 54.6 mN m -1 ) and an emulsification activity index of 95.4%. Characterisation of the biosurfactants produced by the LC-MS/MS method showed the presence of eleven compounds belonging to the mono- and di-rhamnolipids group, most likely produced by P. aeruginosa, which was the most abundant (19.6%) in the community. Importantly, we have found a strong correlation (R = -0.96) of power and biosurfactant activity in response to C/N ratio. This study shows that nitrogen plays an important role in the current-generating metabolism of waste cooking oil. To the best of our knowledge, this is the first study where the nitrogen optimisation was investigated to improve the synthesis of biosurfactants and power generation in a bioelectrochemical system., Competing Interests: Declaration of competing interest 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., (Copyright © 2024 The Author(s). Published by Elsevier Ltd.. All rights reserved.)

Published

2024

16. The influence of benzene on the composition, diversity and performance of the anodic bacterial community in glucose-fed microbial fuel cells.

Author

Tyszkiewicz N, Truu J, Młynarz P, and Pasternak G

Abstract

Bioelectrochemical systems offer unique opportunities to remove recalcitrant environmental pollutants in a net positive energy process, although it remains challenging because of the toxic character of such compounds. In this study, microbial fuel cell (MFC) technology was applied to investigate the benzene degradation process for more than 160 days, where glucose was used as a co-metabolite and a control. We have applied an inoculation strategy that led to the development of 10 individual microbial communities. The electrochemical dynamics of MFC efficiency was observed, along with their 1 H NMR metabolic fingerprints and analysis of the microbial community. The highest power density of 120 mW/m 2 was recorded in the final period of the experiment when benzene/glucose was used as fuel. This is the highest value reported in a benzene/co-substrate system. Metabolite analysis confirmed the full removal of benzene, while the dominance of fermentation products indicated the strong occurrence of non-electrogenic reactions. Based on 16S rRNA gene amplicon sequencing, bacterial community analysis revealed several petroleum-degrading microorganisms, electroactive species and biosurfactant producers. The dominant species were recognised as Citrobacter freundii and Arcobacter faecis . Strong, positive impact of the presence of benzene on the alpha diversity was recorded, underlining the high complexity of the bioelectrochemically supported degradation of petroleum compounds. This study reveals the importance of supporting the bioelectrochemical degradation process with auxiliary substrates and inoculation strategies that allow the communities to reach sufficient diversity to improve the power output and degradation efficiency in MFCs beyond the previously known limits. This study, for the first time, provides an outlook on the syntrophic activity of biosurfactant producers and petroleum degraders towards the efficient removal and conversion of recalcitrant hydrophobic compounds into electricity in MFCs., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest. The author(s) declared that they were an editorial board member of Frontiers, at the time of submission. This had no impact on the peer review process and the final decision., (Copyright © 2024 Tyszkiewicz, Truu, Młynarz and Pasternak.)

Published

2024

17. Glycogen phosphorylase inhibition improves cognitive function of aged mice.

Author

Drulis-Fajdasz D, Krzystyniak A, Puścian A, Pytyś A, Gostomska-Pampuch K, Pudełko-Malik N, Wiśniewski JŁ, Młynarz P, Miazek A, Wójtowicz T, Włodarczyk J, Duś-Szachniewicz K, Gizak A, Wiśniewski JR, and Rakus D

Subjects

Mice, Animals, Memory Disorders metabolism, Cognition, Glycogen metabolism, Dendritic Spines metabolism, Hippocampus metabolism, Glycogen Phosphorylase metabolism

Abstract

Inhibition of glycogen breakdown blocks memory formation in young animals, but it stimulates the maintenance of the long-term potentiation, a cellular mechanism of memory formation, in hippocampal slices of old animals. Here, we report that a 2-week treatment with glycogen phosphorylase inhibitor BAY U6751 alleviated memory deficits and stimulated neuroplasticity in old mice. Using the 2-Novel Object Recognition and Novel Object Location tests, we discovered that the prolonged intraperitoneal administration of BAY U6751 improved memory formation in old mice. This was accompanied by changes in morphology of dendritic spines in hippocampal neurons, and by "rejuvenation" of hippocampal proteome. In contrast, in young animals, inhibition of glycogen degradation impaired memory formation; however, as in old mice, it did not alter significantly the morphology and density of cortical dendritic spines. Our findings provide evidence that prolonged inhibition of glycogen phosphorolysis improves memory formation of old animals. This could lead to the development of new strategies for treatment of age-related memory deficits., (© 2023 The Authors. Aging Cell published by Anatomical Society and John Wiley & Sons Ltd.)

Published

2023

18. The toxicity of nanoparticles and their interaction with cells: an in vitro metabolomic perspective.

Author

Awashra M and Młynarz P

Abstract

Nowadays, nanomaterials (NMs) are widely present in daily life due to their significant benefits, as demonstrated by their application in many fields such as biomedicine, engineering, food, cosmetics, sensing, and energy. However, the increasing production of NMs multiplies the chances of their release into the surrounding environment, making human exposure to NMs inevitable. Currently, nanotoxicology is a crucial field, which focuses on studying the toxicity of NMs. The toxicity or effects of nanoparticles (NPs) on the environment and humans can be preliminary assessed in vitro using cell models. However, the conventional cytotoxicity assays, such as the MTT assay, have some drawbacks including the possibility of interference with the studied NPs. Therefore, it is necessary to employ more advanced techniques that provide high throughput analysis and avoid interferences. In this case, metabolomics is one of the most powerful bioanalytical strategies to assess the toxicity of different materials. By measuring the metabolic change upon the introduction of a stimulus, this technique can reveal the molecular information of the toxicity induced by NPs. This provides the opportunity to design novel and efficient nanodrugs and minimizes the risks of NPs used in industry and other fields. Initially, this review summarizes the ways that NPs and cells interact and the NP parameters that play a role in this interaction, and then the assessment of these interactions using conventional assays and the challenges encountered are discussed. Subsequently, in the main part, we introduce the recent studies employing metabolomics for the assessment of these interactions in vitro ., Competing Interests: There are no conflicts to declare., (This journal is © The Royal Society of Chemistry.)

Published

2023

19. Precision Nutrition in NAFLD: Effects of a High-Fiber Intervention on the Serum Metabolome of NAFD Patients-A Pilot Study.

Author

Stachowska E, Maciejewska-Markiewicz D, Palma J, Mielko KA, Qasem B, Kozłowska-Petriczko K, Ufnal M, Sokolowska KE, Hawryłkowicz V, Załęska P, Jakubczyk K, Wunsch E, Ryterska K, Skonieczna-Żydecka K, and Młynarz P

Subjects

Adult, Humans, Pilot Projects, Nutritional Status, Diet, Metabolome, Non-alcoholic Fatty Liver Disease metabolism

Abstract

Non-alcoholic fatty liver disease (NAFLD) is associated with dysfunction of the intestinal microbiota and its metabolites. We aimed to assess whether replacing bread with high-fiber buns beneficially changes the metabolome in NAFLD patients. This study involved 27 adult patients with NAFLD validated by FibroScan ® (CAP ≥ 234 dB/m). Patients were asked to replace their existing bread for two meals with high-fiber buns. In this way, the patients ate two rolls every day for 2 months. The following parameters were analysed (at the beginning and after 2 months): the anthropometric data (BIA), eating habits (24 h food recalls), gut barrier markers (lipopolysaccharide S and liposaccharide binding protein (LPS, LBP)), serum short-chain fatty acids (SCFAs) and branched chain fatty acids (BCFAs) by GC/MS chromatography, as well as serum metabolites (by 1 H NMR spectroscopy). After 2 months of high-fiber roll consumption, the reduction of liver steatosis was observed (change Fibroscan CAP values from 309-277 dB/m). In serum propionate, acetate, isovaleric, and 2-methylbutyric decrease was observed. Proline, choline and one unknown molecule had higher relative concentration in serum at endpoint. A fiber-targeted dietary approach may be helpful in the treatment of patients with NAFLD, by changing the serum microbiota metabolome.

Published

2022

20. Hydrogel Alginate Seed Coating as an Innovative Method for Delivering Nutrients at the Early Stages of Plant Growth.

Author

Skrzypczak D, Jarzembowski Ł, Izydorczyk G, Mikula K, Hoppe V, Mielko KA, Pudełko-Malik N, Młynarz P, Chojnacka K, and Witek-Krowiak A

Abstract

Seed coating containing fertilizer nutrients and plant growth biostimulants is an innovative technique for precision agriculture. Nutrient delivery can also be conducted through multilayer seed coating. For this purpose, sodium alginate with NPK, which was selected in a preliminary selection study, crosslinked with divalent ions (Cu(II), Mn(II), Zn(II)) as a source of fertilizer micronutrients, was used to produce seed coating. The seeds were additionally coated with a solution containing amino acids derived from high-protein material. Amino acids can be obtained by alkaline hydrolysis of mealworm larvae (Gly 71.2 ± 0.6 mM, Glu 55.8 ± 1.3 mM, Pro 48.8 ± 1.5 mM, Ser 31.4 ± 1.5 mM). The formulations were applied in different doses per 100 g of seeds: 35 mL, 70 mL, 105 mL, and 140 mL. SEM-EDX surface analysis showed that 70 mL of formulation/100 g of seeds formed a continuity of coatings but did not result in a uniform distribution of components on the surface. Extraction tests proved simultaneous low leaching of nutrients into water (max. 10%), showing a slow release pattern. There occurred high bioavailability of fertilizer nutrients (even up to 100%). Pot tests on cucumbers ( Cornichon de Paris ) confirmed the new method's effectiveness, yielding a 50% higher fresh sprout weight and four times greater root length than uncoated seeds. Seed coating with hydrogel has a high potential for commercial application, stimulating the early growth of plants and thus leading to higher crop yields.

Published

2021

21. Effect of 6-Month Feeding with a Diet Enriched in EPA + DHA from Fish Meat on the Blood Metabolomic Profile of Dogs with Myxomatous Mitral Valve Disease.

Author

Pasławski R, Kurosad A, Ząbek A, Pasławska U, Noszczyk-Nowak A, Michałek M, and Młynarz P

Abstract

Animal nutrition plays an important role in the therapy of many diseases, including heart failure. The aim was to assess whether 6 months of feeding an AEP + ADH enriched diet (from fish meat) in dogs suffering from heart failure due to mitral degeneration impacts the dogs' metabolic profile and clinical status. Twenty small breed dogs were included: 50% were in stage B2 of MMVD and 50%, in stage C according to ACVIM. Dogs were randomly divided into two groups. One group receiving a standard diet, the second one a diet enriched with EPA + DHA (from fish meat). All dogs continued to receive appropriate therapy throughout the study. Control examinations were performed at the start of the study, after 3 and 6 months of appropriate feeding. Examinations included ECG, ECHO, blood hemathology and biochemistry, morphometric measurements, body fat index and subcutaneous fat tissue thickness. Serum samples were analyzed with a high-performance liquid chromatography system. Data were analyzed using the Progenesis QI (PQI, Non-linear Dynamics). The results showed no differences in clinical, cardiological, haematological and biochemical parameters between the two study groups. An effect on the metabolomic profile following a continued diet enriched in DHA + EPA (from fish meat) was more pronounced with time. After 6 months of feeding the diete enriched with DHA + EPA (from fish meat), there was a favorable reduction in glycerophosphocholine and xanthine levels, but an adverse increase in lactate and furvan and a decrease in alanine was not stopped.

Published

2021

22. Gender-Specific Metabolomics Approach to Kidney Cancer.

Author

Deja S, Litarski A, Mielko KA, Pudełko-Malik N, Wojtowicz W, Zabek A, Szydełko T, and Młynarz P

Abstract

Renal cell carcinoma (RCC) is the most common form of kidney malignancy. RCC is more common among men with a 2/1 male/female incidence ratio worldwide. Given the underlying epidemiological differences in the RCC incidence between males and females, we explored the gender specific 1 H NMR serum metabolic profiles of RCC patients and their matched controls. A number of differential metabolites were shared by male and female RCC patients. These RCC specific changes included lower lactate, threonine, histidine, and choline levels together with increased levels of pyruvate, N -acetylated glycoproteins, beta-hydroxybutyrate, acetoacetate, and lysine. Additionally, serum lactate/pyruvate ratio was a strong predictor of RCC status regardless of gender. Although only moderate changes in metabolic profiles were observed between control males and females there were substantial gender related differences among RCC patients. Gender specific metabolic features associated with RCC status were identified suggesting that different metabolic panels could be leveraged for a more precise diagnostic.

Published

2021

23. Metabolomics Comparison of Drug-Resistant and Drug-Susceptible Pseudomonas aeruginosa Strain (Intra- and Extracellular Analysis).

Author

Mielko KA, Jabłoński SJ, Pruss Ł, Milczewska J, Sands D, Łukaszewicz M, and Młynarz P

Subjects

Humans, Pseudomonas Infections drug therapy, Pseudomonas Infections microbiology, Pseudomonas aeruginosa drug effects, Pseudomonas aeruginosa isolation & purification, Anti-Bacterial Agents pharmacology, Drug Resistance, Multiple, Bacterial, Metabolome drug effects, Pseudomonas Infections metabolism, Pseudomonas aeruginosa metabolism

Abstract

Pseudomonas aeruginosa is a common human pathogen belonging to the ESKAPE group. The multidrug resistance of bacteria is a considerable problem in treating patients and may lead to increased morbidity and mortality rate. The natural resistance in these organisms is caused by the production of specific enzymes and biofilm formation, while acquired resistance is multifactorial. Precise recognition of potential antibiotic resistance on different molecular levels is essential. Metabolomics tools may aid in the observation of the flux of low molecular weight compounds in biochemical pathways yielding additional information about drug-resistant bacteria. In this study, the metabolisms of two P. aeruginosa strains were compared-antibiotic susceptible vs. resistant. Analysis was performed on both intra- and extracellular metabolites. The 1 H NMR method was used together with multivariate and univariate data analysis, additionally analysis of the metabolic pathways with the FELLA package was performed. The results revealed the differences in P. aeruginosa metabolism of drug-resistant and drug-susceptible strains and provided direct molecular information about P. aeruginosa response for different types of antibiotics. The most significant differences were found in the turnover of amino acids. This study can be a valuable source of information to complement research on drug resistance in P. aeruginosa .

Published

2021

24. Disease Differentiation and Monitoring of Anti-TNF Treatment in Rheumatoid Arthritis and Spondyloarthropathies.

Author

Bogunia-Kubik K, Wojtowicz W, Swierkot J, Mielko KA, Qasem B, Wielińska J, Sokolik R, Pruss Ł, and Młynarz P

Subjects

Adult, Arthritis, Psoriatic drug therapy, Arthritis, Rheumatoid drug therapy, Cohort Studies, Computational Biology, Female, Humans, Magnetic Resonance Spectroscopy, Male, Metabolome, Principal Component Analysis, Spondylitis, Ankylosing drug therapy, Arthritis, Psoriatic blood, Arthritis, Rheumatoid blood, Ethanol blood, Spondylitis, Ankylosing blood, Tumor Necrosis Factor Inhibitors therapeutic use

Abstract

Rheumatoid arthritis (RA), ankylosing spondylitis (AS), and psoriatic arthritis (PsA) are comprehensive immunological disorders. The treatment of these disorders is limited to ameliorating the symptoms and improving the quality of life of patients. In this study, serum samples from RA, AS, and PsA patients were analyzed with metabolomic tools employing the 1H NMR method in combination with univariate and multivariate analyses. The results obtained in this study showed that the changes in metabolites were the highest for AS > RA > PsA. The study demonstrated that the time until remission or until low disease activity is achieved is shortest (approximately three months) for AS, longer for RA and longest for PsA. The statistically common metabolite that was found to be negatively correlated with the healing processes of these disorders is ethanol, which may indicate the involvement of the gut microflora and/or the breakdown of malondialdehyde as a cell membrane lipid peroxide product.

Published

2021

25. Effect of Protoberberine-Rich Fraction of Chelidonium majus L. on Endometriosis Regression.

Author

Warowicka A, Qasem B, Dera-Szymanowska A, Wołuń-Cholewa M, Florczak P, Horst N, Napierała M, Szymanowski K, Popenda Ł, Bartkowiak G, Florek E, Goździcka-Józefiak A, and Młynarz P

Abstract

Endometriosis is a gynecological disease defined by the presence of endometrial tissue outside the uterus. To date, the effective treatment of this disease is still based on invasive surgery or laparoscopy. Chelidonium majus L. (Papaveraceae) belongs to medicinal, latex-bearing plants. Extracts from the plant are a rich source of pharmacologically active agents. Protoberberine compounds derived from C. majus possess anticancer and antiproliferative activities. In the present study of a rat model of endometriosis, we investigated the influence of the plant protoberberine-rich fraction (BBR) obtained from the medicinal plant C. majus on the development of endometriosis. To understand of BBR therapeutic potential for endometriosis, metabolomics has been applied to study. BBR was prepared from an ethanolic extract of dry plants C. majus . Rats ( n = 16) with confirmed endometriosis were treated with BBR administered orally (1 g/kg) for 14 days. Blood serum samples were collected from all of the animals and metabolites were studied using the NMR method. The metabolomic pattern was compared before and after the protoberberine treatment. The performed analysis showed significant changes in the concentrations of metabolites that are involved in energy homeostasis, including glucose, glutamine, and lactate. Histopathological studies showed no recurrence of endometriosis loci after treatment with BBR. The results of the study found that BBR treatment prevents the recurrence of endometriosis in rats. Moreover, metabolomics profiling can be applied to better understand the mechanisms of action of these protoberberine secondary plant metabolites. Our findings provide new insights into the pharmaceutical activity of natural protoberberine plant compounds.

Published

2021

26. An Optimization of Liquid-Liquid Extraction of Urinary Volatile and Semi-Volatile Compounds and Its Application for Gas Chromatography-Mass Spectrometry and Proton Nuclear Magnetic Resonance Spectroscopy.

Author

Drabińska N, Młynarz P, de Lacy Costello B, Jones P, Mielko K, Mielnik J, Persad R, and Ratcliffe NM

Subjects

Female, Humans, Gas Chromatography-Mass Spectrometry methods, Liquid-Liquid Extraction methods, Liquid-Liquid Extraction standards, Proton Magnetic Resonance Spectroscopy methods, Urinalysis methods, Volatile Organic Compounds urine

Abstract

Urinary volatile compounds (VCs) have been recently assessed for disease diagnoses. They belong to very diverse chemical classes, and they are characterized by different volatilities, polarities and concentrations, complicating their analysis via a single analytical procedure. There remains a need for better, lower-cost methods for VC biomarker discovery. Thus, there is a strong need for alternative methods, enabling the detection of a broader range of VCs. Therefore, the main aim of this study was to optimize a simple and reliable liquid-liquid extraction (LLE) procedure for the analysis of VCs in urine using gas chromatography-mass spectrometry (GC-MS), in order to obtain the maximum number of responses. Extraction parameters such as pH, type of solvent and ionic strength were optimized. Moreover, the same extracts were analyzed using Proton Nuclear Magnetic Resonance Spectroscopy ( 1 H-NMR), to evaluate the applicability of a single urine extraction for multiplatform purposes. After the evaluation of experimental conditions, an LLE protocol using 2 mL of urine in the presence of 2 mL of 1 M sulfuric acid and sodium sulphate extracted with dichloromethane was found to be optimal. The optimized method was validated with the external standards and was found to be precise and linear, and allowed for detection of >400 peaks in a single run present in at least 50% of six samples-considerably more than the number of peaks detected by solid-phase microextracton fiber pre-concentration-GC-MS (328 ± 6 vs. 234 ± 4). 1 H-NMR spectroscopy of the polar and non-polar extracts extended the range to >40 more (mainly low volatility compounds) metabolites (non-destructively), the majority of which were different from GC-MS. The more peaks detectable, the greater the opportunity of assessing a fingerprint of several compounds to aid biomarker discovery. In summary, we have successfully demonstrated the potential of LLE as a cheap and simple alternative for the analysis of VCs in urine, and for the first time the applicability of a single urine solvent extraction procedure for detecting a wide range of analytes using both GC-MS and 1 H-NMR analysis to enhance putative biomarker detection. The proposed method will simplify the transport between laboratories and storage of samples, as compared to intact urine samples.

Published

2020

27. Imunofan-RDKVYR Peptide-Stimulates Skin Cell Proliferation and Promotes Tissue Repair.

Author

Sawicka J, Dzierżyńska M, Wardowska A, Deptuła M, Rogujski P, Sosnowski P, Filipowicz N, Mieczkowska A, Sass P, Pawlik A, Hać A, Schumacher A, Gucwa M, Karska N, Kamińska J, Płatek R, Mazuryk J, Zieliński J, Kondej K, Młynarz P, Mucha P, Skowron P, Janus Ł, Herman-Antosiewicz A, Sachadyn P, Czupryn A, Piotrowski A, Pikuła M, and Rodziewicz-Motowidło S

Subjects

Albumins metabolism, Animals, Basophils drug effects, Cell Death drug effects, Cell Line, Chemotaxis drug effects, Cytokines metabolism, DNA Methylation drug effects, Ear pathology, Fibroblasts cytology, Fibroblasts drug effects, HaCaT Cells cytology, HaCaT Cells drug effects, Humans, Injections, Subcutaneous, Mice, Inbred BALB C, Mice, Inbred C57BL, Oligopeptides blood, Oligopeptides chemistry, Oligopeptides metabolism, Protein Stability drug effects, Stem Cells cytology, Stem Cells drug effects, Transcription, Genetic drug effects, Cell Proliferation drug effects, Oligopeptides pharmacology, Skin pathology, Wound Healing

Abstract

Regeneration and wound healing are vital to tissue homeostasis and organism survival. One of the biggest challenges of today's science and medicine is finding methods and factors to stimulate these processes in the human body. Effective solutions to promote regenerative responses will accelerate advances in tissue engineering, regenerative medicine, transplantology, and a number of other clinical specialties. In this study, we assessed the potential efficacy of a synthetic hexapeptide, RDKVYR, for the stimulation of tissue repair and wound healing. The hexapeptide is marketed under the name "Imunofan" (IM) as an immunostimulant. IM displayed stability in aqueous solutions, while in plasma it was rapidly bound by albumins. Structural analyses demonstrated the conformational flexibility of the peptide. Tests in human fibroblast and keratinocyte cell lines showed that IM exerted a statistically significant ( p < 0.05) pro-proliferative activity (30-40% and 20-50% increase in proliferation of fibroblast and keratinocytes, respectively), revealed no cytotoxicity over a vast range of concentrations ( p < 0.05), and had no allergic properties. IM was found to induce significant transcriptional responses, such as enhanced activity of genes involved in active DNA demethylation ( p < 0.05) in fibroblasts and activation of genes involved in immune responses, migration, and chemotaxis in adipose-derived stem cells derived from surgery donors. Experiments in a model of ear pinna injury in mice indicated that IM moderately promoted tissue repair (8% in BALB/c and 36% in C57BL/6 in comparison to control).

Published

2020

28. LC-QTOF-MS and 1 H NMR Metabolomics Verifies Potential Use of Greater Omentum for Klebsiella pneumoniae Biofilm Eradication in Rats.

Author

Teul J, Deja S, Celińska-Janowicz K, Ząbek A, Młynarz P, Barć P, Junka A, Smutnicka D, Bartoszewicz M, Pałka J, and Miltyk W

Abstract

Bacterial wound infections are a common problem associated with surgical interventions. In particular, biofilm-forming bacteria are hard to eradicate, and alternative methods of treatment based on covering wounds with vascularized flaps of tissue are being developed. The greater omentum is a complex organ covering the intestines in the abdomen, which support wound recovery following surgical procedures and exhibit natural antimicrobial activity that could improve biofilm eradication. We investigated changes in rats' metabolome following Klebsiella pneumoniae infections, as well as the greater omentum's ability for Klebsiella pneumoniae biofilm eradication. Rats received either sterile implants or implants covered with Klebsiella pneumoniae biofilm (placed in the peritoneum or greater omentum). Metabolic profiles were monitored at days 0, 2, and 5 after surgery using combined proton nuclear magnetic resonance ( 1 H NMR) and high performance liquid chromatography quadrupole time-of-flight tandem mass spectrometry (LC-QTOF‑MS) measurements of urine samples followed by chemometric analysis. Obtained results indicated that grafting of the sterile implant to the greater omentum did not cause major disturbances in rats' metabolism, whereas the sterile implant located in the peritoneum triggered metabolic perturbations related to tricarboxylic acid (TCA) cycle, as well as choline, tryptophan, and hippurate metabolism. Presence of implants colonized with Klebsiella pneumoniae biofilm resulted in similar levels of metabolic perturbations in both locations. Our findings confirmed that surgical procedures utilizing the greater omentum may have a practical use in wound healing and tissue regeneration in the future.

Published

2020

29. Evaluation of MDA-MB-468 Cell Culture Media Analysis in Predicting Triple-Negative Breast Cancer Patient Sera Metabolic Profiles.

Author

Wojtowicz W, Wróbel A, Pyziak K, Tarkowski R, Balcerzak A, Bębenek M, and Młynarz P

Abstract

Triple-negative breast cancer (TNBC) is characterized by limited survival, poor prognosis, and high recurrence. Understanding the metabolic adaptations of TNBC could help reveal improved treatment regiments. Here we performed a comprehensive 1 H NMR metabolic characterization of the MDA-MB-468 cell line, a commonly used model of TNBC, followed by an analysis of serum samples obtained from TNBC patients and healthy controls. MDA-MB-468 cells were cultured, and changes in the metabolic composition of the medium were monitored for 72 h. Based on time courses, metabolites were categorized as being consumed, being produced, or showing a mixed behavior. When comparing TNBC and control samples (HC), and by using multivariate and univariate analyses, we identified nine metabolites with differing profiles). The serum of TNBC patients was characterized by higher levels of glucose, glutamine, citrate, and acetoacetate and by lower levels of lactate, alanine, tyrosine, glutamate, and acetone. A comparative analysis between MDA-MB-468 cell culture media and TNBC patients' serum identified a potential systemic response to the carcinogenesis-associated processes, highlighting that MDA-MB-468 cells footprint does not reflect metabolic changes observed in studied TNBC serum fingerprint., Competing Interests: The authors declare that they have no competing interests.

Published

2020

30. Serine Biosynthesis Pathway Supports MYC-miR-494-EZH2 Feed-Forward Circuit Necessary to Maintain Metabolic and Epigenetic Reprogramming of Burkitt Lymphoma Cells.

Author

Białopiotrowicz E, Noyszewska-Kania M, Kachamakova-Trojanowska N, Łoboda A, Cybulska M, Grochowska A, Kopczyński M, Mikula M, Prochorec-Sobieszek M, Firczuk M, Graczyk-Jarzynka A, Zagożdżon R, Ząbek A, Młynarz P, Dulak J, Górniak P, Szydłowski M, Pyziak K, Martyka J, Sroka-Porada A, Jabłońska E, Polak A, Kowalczyk P, Szumera-Ciećkiewicz A, Chapuy B, Rzymski T, Brzózka K, and Juszczyński P

Abstract

Burkitt lymphoma (BL) is a rapidly growing tumor, characterized by high anabolic requirements. The MYC oncogene plays a central role in the pathogenesis of this malignancy, controlling genes involved in apoptosis, proliferation, and cellular metabolism. Serine biosynthesis pathway (SBP) couples glycolysis to folate and methionine cycles, supporting biosynthesis of certain amino acids, nucleotides, glutathione, and a methyl group donor, S-adenosylmethionine (SAM). We report that BLs overexpress SBP enzymes, phosphoglycerate dehydrogenase (PHGDH) and phosphoserine aminotransferase 1 (PSAT1). Both genes are controlled by the MYC-dependent ATF4 transcription factor. Genetic ablation of PHGDH/PSAT1 or chemical PHGDH inhibition with NCT-503 decreased BL cell lines proliferation and clonogenicity. NCT-503 reduced glutathione level, increased reactive oxygen species abundance, and induced apoptosis. Consistent with the role of SAM as a methyl donor, NCT-503 decreased DNA and histone methylation, and led to the re-expression of ID4 , KLF4 , CDKN2B and TXNIP tumor suppressors. High H3K27me3 level is known to repress the MYC negative regulator miR-494. NCT-503 decreased H3K27me3 abundance, increased the miR-494 level, and reduced the expression of MYC and MYC-dependent histone methyltransferase, EZH2. Surprisingly, chemical/genetic disruption of SBP did not delay BL and breast cancer xenografts growth, suggesting the existence of mechanisms compensating the PHGDH/PSAT1 absence in vivo., Competing Interests: P. Juszczynski is a member of the Scientific Advisory Board at Selvita S.A. and served as a consultant for Selvita S.A. Dr. T. Rzymski, Dr. K. Brzozka and P. Kowalczyk are Selvita S.A. employees.

Published

2020

31. N-phosphonomethylglycine utilization by the psychrotolerant yeast Solicoccozyma terricola M 3.1.4.

Author

Stosiek N, Terebieniec A, Ząbek A, Młynarz P, Cieśliński H, and Klimek-Ochab M

Subjects

DNA, Fungal, Glycine chemistry, Organophosphonates metabolism, Oxidoreductases metabolism, Phosphorus metabolism, Phylogeny, Yeasts genetics, Glyphosate, Glycine analogs & derivatives, Glycine metabolism, Yeasts metabolism

Abstract

Solicoccozyma terricola M 3.1.4., the yeast strain isolated from soil sample from blueberry cultivation in Miedzyrzec Podlaski in Poland, is capable to split of phosphorus to nitrogen and nitrogen to carbon bonds in N-phosphonomethylglycine (PMG, glyphosate). The biodegradation process proceeds in the phosphate-independent manner. It is the first example of a psychrotolerant yeast strain able to degrade PMG via CN bond cleavage accompanied by AMPA formation and not like in most microorganisms via CP bond disruption followed by the sarcosine pathway. Glyphosate oxidoreductase (GOX) type activity was detected in cell-free extracts prepared from S. terricola M 3.1.4. pregrown on 4 mM PMG as a sole phosphorus and nitrogen source in cultivation medium., (Copyright © 2019 Elsevier Inc. All rights reserved.)

Published

2019

32. Serum NMR metabolomics to differentiate haematologic malignancies.

Author

Wojtowicz W, Chachaj A, Olczak A, Ząbek A, Piątkowska E, Rybka J, Butrym A, Biedroń M, Mazur G, Wróbel T, Szuba A, and Młynarz P

Abstract

Haematological malignancies are a frequently diagnosed group of neoplasms and a significant cause of cancer deaths. The successful treatment of these diseases relies on early and accurate detection. Specific small molecular compounds released by malignant cells and the simultaneous response by the organism towards the pathological state may serve as diagnostic/prognostic biomarkers or as a tool with relevance for cancer therapy management. To identify the most important metabolites required for differentiation, an 1 H NMR metabolomics approach was applied to selected haematological malignancies. This study utilized 116 methanol serum extract samples from AML (n= 38), nHL (n= 26), CLL (n= 21) and HC (n= 31). Multivariate and univariate data analyses were performed to identify the most abundant changes among the studied groups. Complex and detailed VIP-PLS-DA models were calculated to highlight possible changes in terms of biochemical pathways and discrimination ability. Chemometric model prediction properties were validated by receiver operating characteristic (ROC) curves and statistical analysis. Two sets of eight important metabolites in HC/AML/CLL/nHL comparisons and five in AML/CLL/nHL comparisons were selected to form complex models to represent the most significant changes that occurred., Competing Interests: CONFLICTS OF INTEREST The authors declare that they have no competing interests.

Published

2018

33. Photochromic switching of the DNA helicity induced by azobenzene derivatives.

Author

Deiana M, Pokladek Z, Olesiak-Banska J, Młynarz P, Samoc M, and Matczyszyn K

Subjects

Light, Photochemistry methods, Protein Structure, Secondary, Azo Compounds chemistry, DNA, B-Form chemistry

Abstract

The photochromic properties of azobenzene, involving conformational changes occurring upon interaction with light, provide an excellent tool to establish new ways of selective regulation applied to biosystems. We report here on the binding of two water-soluble 4-(phenylazo)benzoic acid derivatives (Azo-2N and Azo-3N) with double stranded DNA and demonstrate that the photoisomerization of Azo-3N leads to changes in DNA structure. In particular, we show that stabilization and destabilization of the B-DNA secondary structure can be photochemically induced in situ by light. This photo-triggered process is fully reversible and could be an alternative pathway to control a broad range of biological processes. Moreover, we found that the bicationic Azo-3N exhibited a higher DNA-binding constant than the monocationic Azo-2N pointing out that the number of positive charges along the photosensitive polyamines chain plays a pivotal role in stabilizing the photochrome-DNA complex.

Published

2016

34. 1H NMR-based metabolic profiling for evaluating poppy seed rancidity and brewing.

Author

Jawień E, Ząbek A, Deja S, Łukaszewicz M, and Młynarz P

Subjects

Biomarkers metabolism, Discriminant Analysis, Germination, Papaver chemistry, Principal Component Analysis, Seeds chemistry, Seeds metabolism, Temperature, Metabolome, Papaver metabolism, Proton Magnetic Resonance Spectroscopy

Abstract

Poppy seeds are widely used in household and commercial confectionery. The aim of this study was to demonstrate the application of metabolic profiling for industrial monitoring of the molecular changes which occur during minced poppy seed rancidity and brewing processes performed on raw seeds. Both forms of poppy seeds were obtained from a confectionery company. Proton nuclear magnetic resonance (1H NMR) was applied as the analytical method of choice together with multivariate statistical data analysis. Metabolic fingerprinting was applied as a bioprocess control tool to monitor rancidity with the trajectory of change and brewing progressions. Low molecular weight compounds were found to be statistically significant biomarkers of these bioprocesses. Changes in concentrations of chemical compounds were explained relative to the biochemical processes and external conditions. The obtained results provide valuable and comprehensive information to gain a better understanding of the biology of rancidity and brewing processes, while demonstrating the potential for applying NMR spectroscopy combined with multivariate data analysis tools for quality control in food industries involved in the processing of oilseeds. This precious and versatile information gives a better understanding of the biology of these processes.

Published

2015

35. Do differences in chemical composition of stem and cap of Amanita muscaria fruiting bodies correlate with topsoil type?

Author

Deja S, Wieczorek PP, Halama M, Jasicka-Misiak I, Kafarski P, Poliwoda A, and Młynarz P

Subjects

Ecosystem, Amanita chemistry, Amanita metabolism, Fruiting Bodies, Fungal chemistry, Fruiting Bodies, Fungal metabolism, Soil chemistry

Abstract

Fly agaric (Amanita muscaria) was investigated using a 1H NMR-based metabolomics approach. The caps and stems were studied separately, revealing different metabolic compositions. Additionally, multivariate data analyses of the fungal basidiomata and the type of soil were performed. Compared to the stems, A. muscaria caps exhibited higher concentrations of isoleucine, leucine, valine, alanine, aspartate, asparagine, threonine, lipids (mainly free fatty acids), choline, glycerophosphocholine (GPC), acetate, adenosine, uridine, 4-aminobutyrate, 6-hydroxynicotinate, quinolinate, UDP-carbohydrate and glycerol. Conversely, they exhibited lower concentrations of formate, fumarate, trehalose, α- and β-glucose. Six metabolites, malate, succinate, gluconate, N-acetylated compounds (NAC), tyrosine and phenylalanine, were detected in whole A. muscaria fruiting bodies but did not show significant differences in their levels between caps and stems (P value>0.05 and/or OPLS-DA loading correlation coefficient <0.4). This methodology allowed for the differentiation between the fruiting bodies of A. muscaria from mineral and mineral-organic topsoil. Moreover, the metabolomic approach and multivariate tools enabled to ascribe the basidiomata of fly agaric to the type of topsoil. Obtained results revealed that stems metabolome is more dependent on the topsoil type than caps. The correlation between metabolites and topsoil contents together with its properties exhibited mutual dependences.

Published

2014

36. Synthesis of fluorescent (benzyloxycarbonylamino)(aryl)methylphosphonates.

Author

Górniak MG, Czernicka A, Młynarz P, Balcerzak W, and Kafarski P

Abstract

The synthesis of a library of structurally variable aromatic esters of (benzyloxycarbonylamino)(aryl)methylphosphonic acids is described by means of the Oleksyszyn reaction. The library was enlarged by the application of a Suzuki-Miayra approach and by preparation of mixed esters.

Published

2014

37. Serum and urine metabolomic fingerprinting in diagnostics of inflammatory bowel diseases.

Author

Dawiskiba T, Deja S, Mulak A, Ząbek A, Jawień E, Pawełka D, Banasik M, Mastalerz-Migas A, Balcerzak W, Kaliszewski K, Skóra J, Barć P, Korta K, Pormańczuk K, Szyber P, Litarski A, and Młynarz P

Subjects

Adolescent, Adult, Aged, Area Under Curve, Biomarkers blood, Biomarkers urine, Case-Control Studies, Colitis, Ulcerative blood, Colitis, Ulcerative therapy, Colitis, Ulcerative urine, Crohn Disease blood, Crohn Disease therapy, Crohn Disease urine, Diagnosis, Differential, Discriminant Analysis, Female, Humans, Least-Squares Analysis, Magnetic Resonance Spectroscopy, Male, Middle Aged, Poland, Predictive Value of Tests, Prognosis, ROC Curve, Remission Induction, Severity of Illness Index, Young Adult, Colitis, Ulcerative diagnosis, Crohn Disease diagnosis, Metabolomics methods

Abstract

Aim: To evaluate the utility of serum and urine metabolomic analysis in diagnosing and monitoring of inflammatory bowel diseases (IBD)., Methods: Serum and urine samples were collected from 24 patients with ulcerative colitis (UC), 19 patients with the Crohn's disease (CD) and 17 healthy controls. The activity of UC was assessed with the Simple Clinical Colitis Activity Index, while the activity of CD was determined using the Harvey-Bradshaw Index. The analysis of serum and urine samples was performed using proton nuclear magnetic resonance (NMR) spectroscopy. All spectra were exported to Matlab for preprocessing which resulted in two data matrixes for serum and urine. Prior to the chemometric analysis, both data sets were unit variance scaled. The differences in metabolite fingerprints were assessed using partial least-squares-discriminant analysis (PLS-DA). Receiver operating characteristic curves and area under curves were used to evaluate the quality and prediction performance of the obtained PLS-DA models. Metabolites responsible for separation in models were tested using STATISTICA 10 with the Mann-Whitney-Wilcoxon test and the Student's t test (α = 0.05)., Results: The comparison between the group of patients with active IBD and the group with IBD in remission provided good PLS-DA models (P value 0.002 for serum and 0.003 for urine). The metabolites that allowed to distinguish these groups were: N-acetylated compounds and phenylalanine (up-regulated in serum), low-density lipoproteins and very low-density lipoproteins (decreased in serum) as well as glycine (increased in urine) and acetoacetate (decreased in urine). The significant differences in metabolomic profiles were also found between the group of patients with active IBD and healthy control subjects providing the PLS-DA models with a very good separation (P value < 0.001 for serum and 0.003 for urine). The metabolites that were found to be the strongest biomarkers included in this case: leucine, isoleucine, 3-hydroxybutyric acid, N-acetylated compounds, acetoacetate, glycine, phenylalanine and lactate (increased in serum), creatine, dimethyl sulfone, histidine, choline and its derivatives (decreased in serum), as well as citrate, hippurate, trigonelline, taurine, succinate and 2-hydroxyisobutyrate (decreased in urine). No clear separation in PLS-DA models was found between CD and UC patients based on the analysis of serum and urine samples, although one metabolite (formate) in univariate statistical analysis was significantly lower in serum of patients with active CD, and two metabolites (alanine and N-acetylated compounds) were significantly higher in serum of patients with CD when comparing jointly patients in the remission and active phase of the diseases. Contrary to the results obtained from the serum samples, the analysis of urine samples allowed to distinguish patients with IBD in remission from healthy control subjects. The metabolites of importance included in this case up-regulated acetoacetate and down-regulated citrate, hippurate, taurine, succinate, glycine, alanine and formate., Conclusion: NMR-based metabolomic fingerprinting of serum and urine has the potential to be a useful tool in distinguishing patients with active IBD from those in remission.

Published

2014

38. Follicular adenomas exhibit a unique metabolic profile. ¹H NMR studies of thyroid lesions.

Author

Deja S, Dawiskiba T, Balcerzak W, Orczyk-Pawiłowicz M, Głód M, Pawełka D, and Młynarz P

Subjects

Humans, Magnetic Resonance Spectroscopy, Multivariate Analysis, Adenoma diagnosis, Adenoma metabolism, Biomarkers, Tumor metabolism, Metabolomics methods, Thyroid Neoplasms diagnosis, Thyroid Neoplasms metabolism

Abstract

Thyroid cancer is the most common endocrine malignancy. However, more than 90% of thyroid nodules are benign. It remains unclear whether thyroid carcinoma arises from preexisting benign nodules. Metabolomics can provide valuable and comprehensive information about low molecular weight compounds present in living systems and further our understanding of the biology regulating pathological processes. Herein, we applied ¹H NMR-based metabolic profiling to identify the metabolites present in aqueous tissue extracts of healthy thyroid tissue (H), non-neoplastic nodules (NN), follicular adenomas (FA) and malignant thyroid cancer (TC) as an alternative way of investigating cancer lesions. Multivariate statistical methods provided clear discrimination not only between healthy thyroid tissue and pathological thyroid tissue but also between different types of thyroid lesions. Potential biomarkers common to all thyroid lesions were identified, namely, alanine, methionine, acetone, glutamate, glycine, lactate, tyrosine, phenylalanine and hypoxanthine. Metabolic changes in thyroid cancer were mainly related to osmotic regulators (taurine and scyllo- and myo-inositol), citrate, and amino acids supplying the TCA cycle. Thyroid follicular adenomas were found to display metabolic features of benign non-neoplastic nodules and simultaneously displayed a partial metabolic profile associated with malignancy. This finding allows the discrimination of follicular adenomas from benign non-neoplastic nodules and thyroid cancer with similar accuracy. Moreover, the presented data indicate that follicular adenoma could be an individual stage of thyroid cancer development.

Published

2013

39. Differences in metabolic profiles of planktonic and biofilm cells in Staphylococcus aureus - (1)H Nuclear Magnetic Resonance search for candidate biomarkers.

Author

Junka AF, Deja S, Smutnicka D, Szymczyk P, Ziółkowski G, Bartoszewicz M, and Młynarz P

Subjects

Alanine isolation & purification, Alanine metabolism, Biomarkers metabolism, Butylene Glycols isolation & purification, Butylene Glycols metabolism, Hydrogen, Isoleucine isolation & purification, Isoleucine metabolism, Magnetic Resonance Spectroscopy, Radioisotopes, Staphylococcal Infections microbiology, Staphylococcus aureus growth & development, Staphylococcus aureus isolation & purification, Tomography, X-Ray Computed, Biofilms growth & development, Metabolome, Staphylococcal Infections diagnosis, Staphylococcus aureus metabolism

Abstract

Staphylococcus aureus is responsible for many types of infections related to biofilm presence. As the early diagnostics remains the best option for prevention of biofilm infections, the aim of the work presented was to search for differences in metabolite patterns of S. aureus ATCC6538 biofilm vs. free-swimming S. aureus planktonic forms. For this purpose, Nuclear Magnetic Resonance (NMR) spectroscopy was applied. Data obtained were supported by means of Scanning Electron Microscopy, quantitative cultures and X-ray computed microtomography. Metabolic trends accompanying S. aureus biofilm formation were found using Principal Component Analysis (PCA). Levels of isoleucine, alanine and 2,3-butanediol were significantly higher in biofilm than in planktonic forms, whereas level of osmoprotectant glycine-betaine was significantly higher in planktonic forms of S. aureus. Results obtained may find future application in clinical diagnostics of S. aureus biofilm-related infections.

Published

2013