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3. Current methods to analyse lysosome morphology, positioning, motility and function

Author

Barral, Duarte C, Staiano, Leopoldo, Almeida, Cláudia Guimas, Cutler, Dan F, Eden, Emily R, Futter, Clare E, Galione, Antony, Marques, André R A, Medina, Diego Luis, Napolitano, Gennaro, Settembre, Carmine, Vieira, Otília V, Aerts, Johannes M F G, Atakpa-Adaji, Peace, Bruno, Gemma, Capuozzo, Antonella, De Leonibus, Elvira, Di Malta, Chiara, Escrevente, Cristina, Esposito, Alessandra, Grumati, Paolo, Hall, Michael J, Teodoro, Rita O, Lopes, Susana S, Luzio, J Paul, Monfregola, Jlenia, Montefusco, Sandro, Platt, Frances M, Polishuck, Roman, De Risi, Maria, Sambri, Irene, Soldati, Chiara, Seabra, Miguel C, iNOVA4Health - pólo NMS, Centro de Estudos de Doenças Crónicas (CEDOC), and NOVA Medical School|Faculdade de Ciências Médicas (NMS|FCM)

Abstract

Funding: We thank Liliana Bento for valuable assistance in formatting the manuscript. This article was supported by the LYSOCIL project. This project has received funding from the European Union's Horizon 2020 research and innovation programme under grant agreement No 811087. CGA has funding from Maratona da Saúde 2016 and Fundaçao para a Ciência e a Tecnologia ˜ , I.P. (CEECIND/00410/2017). FMP is a Wellcome Investigator in Science and a Royal Society Wilson merit award holder. Since the discovery of lysosomes more than 70 years ago, much has been learned about the functions of these organelles. Lysosomes were regarded as exclusively degradative organelles, but more recent research has revealed that they play essential roles in several other cellular functions, such as nutrient sensing, intracellular signalling, and metabolism. Methodological advances played a key part in generating our current knowledge about the biology of this multifaceted organelle. In this review, we cover current methods used to analyse lysosome morphology, positioning, motility, and function. We highlight the principles behind these methods, the methodological strategies, and their advantages and limitations. To extract accurate information and avoid misinterpretations, we discuss the best strategies to identify lysosomes and assess their characteristics and functions. With this review, we aim to stimulate an increase in the quantity and quality of research on lysosomes and further ground-breaking discoveries on an organelle that continues to surprise and excite cell biologists. publishersversion published

Published
2022

4. Current methods to analyze lysosome morphology, positioning, motility and function

Author

Barral, Duarte C., primary, Staiano, Leopoldo, additional, Guimas Almeida, Cláudia, additional, Cutler, Dan F., additional, Eden, Emily R., additional, Futter, Clare E., additional, Galione, Antony, additional, Marques, André R. A., additional, Medina, Diego Luis, additional, Napolitano, Gennaro, additional, Settembre, Carmine, additional, Vieira, Otília V., additional, Aerts, Johannes M. F. G., additional, Atakpa‐Adaji, Peace, additional, Bruno, Gemma, additional, Capuozzo, Antonella, additional, De Leonibus, Elvira, additional, Di Malta, Chiara, additional, Escrevente, Cristina, additional, Esposito, Alessandra, additional, Grumati, Paolo, additional, Hall, Michael J., additional, Teodoro, Rita O., additional, Lopes, Susana S., additional, Luzio, J. Paul, additional, Monfregola, Jlenia, additional, Montefusco, Sandro, additional, Platt, Frances M., additional, Polishchuck, Roman, additional, De Risi, Maria, additional, Sambri, Irene, additional, Soldati, Chiara, additional, and Seabra, Miguel C., additional

Published
2022
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5. Beclin‐1‐mediated activation of autophagy improves proximal and distal urea cycle disorders

Author

Soria, Leandro R, primary, Gurung, Sonam, additional, De Sabbata, Giulia, additional, Perocheau, Dany P, additional, De Angelis, Angela, additional, Bruno, Gemma, additional, Polishchuk, Elena, additional, Paris, Debora, additional, Cuomo, Paola, additional, Motta, Andrea, additional, Orford, Michael, additional, Khalil, Youssef, additional, Eaton, Simon, additional, Mills, Philippa B, additional, Waddington, Simon N, additional, Settembre, Carmine, additional, Muro, Andrés F, additional, Baruteau, Julien, additional, and Brunetti‐Pierri, Nicola, additional

Published
2020
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6. Beclin-1-mediated activation of autophagy improves proximal and distal urea cycle disorders

Author

Soria, Leandro R., primary, Perocheau, Dany P., additional, De Sabbata, Giulia, additional, De Angelis, Angela, additional, Bruno, Gemma, additional, Polishchuk, Elena, additional, Gurung, Sonam, additional, Paris, Debora, additional, Cuomo, Paola, additional, Motta, Andrea, additional, Orford, Michael, additional, Eaton, Simon, additional, Waddington, Simon, additional, Settembre, Carmine, additional, Muro, Andrés F., additional, Baruteau, Julien, additional, and Brunetti-Pierri, Nicola, additional

Published
2020
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7. A selective ER ‐phagy exerts procollagen quality control via a Calnexin‐ FAM 134B complex

Author

Forrester, Alison, primary, De Leonibus, Chiara, additional, Grumati, Paolo, additional, Fasana, Elisa, additional, Piemontese, Marilina, additional, Staiano, Leopoldo, additional, Fregno, Ilaria, additional, Raimondi, Andrea, additional, Marazza, Alessandro, additional, Bruno, Gemma, additional, Iavazzo, Maria, additional, Intartaglia, Daniela, additional, Seczynska, Marta, additional, Anken, Eelco, additional, Conte, Ivan, additional, De Matteis, Maria Antonietta, additional, Dikic, Ivan, additional, Molinari, Maurizio, additional, and Settembre, Carmine, additional

Published
2018
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8. A selective ER‐phagy exerts procollagen quality control via a Calnexin‐FAM134B complex

Author

Forrester, Alison, De Leonibus, Chiara, Grumati, Paolo, Fasana, Elisa, Piemontese, Marilina, Staiano, Leopoldo, Fregno, Ilaria, Raimondi, Andrea, Marazza, Alessandro, Bruno, Gemma, Iavazzo, Maria, Intartaglia, Daniela, Seczynska, Marta, Anken, Eelco van, Conte, Ivan, De Matteis, Maria Antonietta, Đikić, Ivan, Molinari, Maurizio, Settembre, Carmine, Forrester, Alison, De Leonibus, Chiara, Grumati, Paolo, Fasana, Elisa, Piemontese, Marilina, Staiano, Leopoldo, Fregno, Ilaria, Raimondi, Andrea, Marazza, Alessandro, Bruno, Gemma, Iavazzo, Maria, Intartaglia, Daniela, Seczynska, Marta, Anken, Eelco van, Conte, Ivan, De Matteis, Maria Antonietta, Đikić, Ivan, Molinari, Maurizio, and Settembre, Carmine

Abstract

Autophagy is a cytosolic quality control process that recognizes substrates through receptor‐mediated mechanisms. Procollagens, the most abundant gene products in Metazoa, are synthesized in the endoplasmic reticulum (ER), and a fraction that fails to attain the native structure is cleared by autophagy. However, how autophagy selectively recognizes misfolded procollagens in the ER lumen is still unknown. We performed siRNA interference, CRISPR‐Cas9 or knockout‐mediated gene deletion of candidate autophagy and ER proteins in collagen producing cells. We found that the ER‐resident lectin chaperone Calnexin (CANX) and the ER‐phagy receptor FAM134B are required for autophagy‐mediated quality control of endogenous procollagens. Mechanistically, CANX acts as co‐receptor that recognizes ER luminal misfolded procollagens and interacts with the ER‐phagy receptor FAM134B. In turn, FAM134B binds the autophagosome membrane‐associated protein LC3 and delivers a portion of ER containing both CANX and procollagen to the lysosome for degradation. Thus, a crosstalk between the ER quality control machinery and the autophagy pathway selectively disposes of proteasome‐resistant misfolded clients from the ER.

Published
2018

9. Similar occurrence of febrile episodes reported in non-atopic children at three to five years of age after prebiotics supplemented infant formula

Author

Van Stuijvenberg, Margriet, Stam, José, Grüber, Christoph, Mosca, Fabio, Arslanoglu, Sertac, Chirico, Gaetano, Braegger, Christian P., Riedler, Josef, Boehm, Günther, Sauer, Pieter J J, Van Der Schaaf, Caroline, Wahn, Ulrich, Wauer, Juliane, Parasher, Kirn, Wust, Madeleine, Lawnitzak, Ingrid, Trentmann, Marion, Schulz, Gabi, Hamelmann, Eckard, Paschke-Goossens, Susanne, Bellach, Johanna, Ahrens, Birgit, Roggero, Paola, Piemontese, Pasqua, Gianni, Maria Lorella, Morlacchi, Laura, Moro, Guido, Rizzardi, Silvia, Rigotti, Elisa, Tandoi, Laura, Coppola, Michela, Bühr, Patrick, Friedt, Michael, Koller, Rebecca, Rogler, Daniela, Rueger, Vanessa, Macheiner, Margret, Tyma, Christine, Antonella, Gasparoni, Elena, Garzoli, Chiara, Offer, Vania, Spinoni, Graziella, Iacono, Maria, Stellini, Van Der Mooren, Jan, Yavuz, Yalcin, Garssen, Johan, Knippels, Leon, Knol, Jan, Amor, Kaouther Ben, Jelinek, Jürgen, Stahl, Bernd, König, Esther, Frings, Anja, Wittke, Anja, Zens, Yvonne, Cremers, Stephanie, Friedrichs, Kathrin, Gerloff, Janine, Bruno, Gemma, Fischer, Ayako, Pharmacology, Sub Immunopharmacology, and Sub General Pharmacology

Subjects
Medicine(all), Agricultural and Biological Sciences(all), Biochemistry, Genetics and Molecular Biology(all)
Abstract

This is a follow up study of a multicenter randomised placebo-controlled trial in seven centres in five West European countries. The RCT assessed the effect of infant formula supplemented with a mixture of prebiotics (with neutral short-chain and long-chain oligosaccharides and pectin-derived acidic oligosaccharides) during infancy in term-born children (n=1130). In the follow-up study 672 children (60% of the study population) participated: 232 (56%) from the prebiotics group (PG), 243 (58%) from the control group (CG), and 197 (66%) from the non-randomised breast-fed group (BG). The primary outcome was the occurrence of febrile episodes at three to five years of age prospectively documented by the parents: in the PG 1.17 (interquartile range 0.50-2.08) episodes per year versus 1.20 (0.52-2.57) in the CG; and 1.48 (0.65-2.60) in the BG. This specific prebiotics mixture given during infancy in healthy non-atopic subjects does not decrease febrile episodes and therefore seems not to prevent infection between their third and fifth birthday.

Published
2015

10. Similar occurrence of febrile episodes reported in non-atopic children at three to five years of age after prebiotics supplemented infant formula

Author

Pharmacology, Sub Immunopharmacology, Sub General Pharmacology, Van Stuijvenberg, Margriet, Stam, José, Grüber, Christoph, Mosca, Fabio, Arslanoglu, Sertac, Chirico, Gaetano, Braegger, Christian P., Riedler, Josef, Boehm, Günther, Sauer, Pieter J J, Van Der Schaaf, Caroline, Wahn, Ulrich, Wauer, Juliane, Parasher, Kirn, Wust, Madeleine, Lawnitzak, Ingrid, Trentmann, Marion, Schulz, Gabi, Hamelmann, Eckard, Paschke-Goossens, Susanne, Bellach, Johanna, Ahrens, Birgit, Roggero, Paola, Piemontese, Pasqua, Gianni, Maria Lorella, Morlacchi, Laura, Moro, Guido, Rizzardi, Silvia, Rigotti, Elisa, Tandoi, Laura, Coppola, Michela, Bühr, Patrick, Friedt, Michael, Koller, Rebecca, Rogler, Daniela, Rueger, Vanessa, Macheiner, Margret, Tyma, Christine, Antonella, Gasparoni, Elena, Garzoli, Chiara, Offer, Vania, Spinoni, Graziella, Iacono, Maria, Stellini, Van Der Mooren, Jan, Yavuz, Yalcin, Garssen, Johan, Knippels, Leon, Knol, Jan, Amor, Kaouther Ben, Jelinek, Jürgen, Stahl, Bernd, König, Esther, Frings, Anja, Wittke, Anja, Zens, Yvonne, Cremers, Stephanie, Friedrichs, Kathrin, Gerloff, Janine, Bruno, Gemma, Fischer, Ayako, Pharmacology, Sub Immunopharmacology, Sub General Pharmacology, Van Stuijvenberg, Margriet, Stam, José, Grüber, Christoph, Mosca, Fabio, Arslanoglu, Sertac, Chirico, Gaetano, Braegger, Christian P., Riedler, Josef, Boehm, Günther, Sauer, Pieter J J, Van Der Schaaf, Caroline, Wahn, Ulrich, Wauer, Juliane, Parasher, Kirn, Wust, Madeleine, Lawnitzak, Ingrid, Trentmann, Marion, Schulz, Gabi, Hamelmann, Eckard, Paschke-Goossens, Susanne, Bellach, Johanna, Ahrens, Birgit, Roggero, Paola, Piemontese, Pasqua, Gianni, Maria Lorella, Morlacchi, Laura, Moro, Guido, Rizzardi, Silvia, Rigotti, Elisa, Tandoi, Laura, Coppola, Michela, Bühr, Patrick, Friedt, Michael, Koller, Rebecca, Rogler, Daniela, Rueger, Vanessa, Macheiner, Margret, Tyma, Christine, Antonella, Gasparoni, Elena, Garzoli, Chiara, Offer, Vania, Spinoni, Graziella, Iacono, Maria, Stellini, Van Der Mooren, Jan, Yavuz, Yalcin, Garssen, Johan, Knippels, Leon, Knol, Jan, Amor, Kaouther Ben, Jelinek, Jürgen, Stahl, Bernd, König, Esther, Frings, Anja, Wittke, Anja, Zens, Yvonne, Cremers, Stephanie, Friedrichs, Kathrin, Gerloff, Janine, Bruno, Gemma, and Fischer, Ayako

Published
2015

11. Determinazione di metalli pesanti in acqua, sedimenti e crostacei (Melicertus kerathurus) della laguna di Lesina

Author

D'ADAMO RAFFAELE, FABBROCINI ADELE, SCIROCCO TOMMASO, CASOLINO GIOVANNI, VOLPE MARIA GRAZIA, RATTO ANTONIO, DI STASIO MICHELE, BRUNO GEMMA, PICIOCCHI NATALÌA, and MECCARIELLO CLEMENTE

Abstract

La laguna di Lesina raccoglie le acque ricche di inquinanti di origine agricola provenienti dal bacino idrografico. Infatti, nel bacino imbrifero è praticata un'agricoltura intensiva spesso al limite della sostenibilità con uso massivo di prodotti chimici. Questi prodotti spesso contengono metalli pesanti che possono essere veicolati in laguna per dilavamento dei terreni. Le lagune hanno un' elevata capacità biogenica e la produzione ittica rappresenta la principale fonte di reddito. In laguna sono presenti specie ittiche che occupano diversi livelli trofici, e a diverso velocità di accrescimento. La mazzancolla (Melicertus kerathurus) è una specie che svolge in laguna un breve periodo del suo ciclo vitale, da post-larva a 3-10 g raggiunti a fine estate, poi migra verso il mare. Nel presente lavoro sono stati analizzati, mediante spettrofotometria ad assorbimento atomico, Cr, Cd, Pb, Zn, Mn e Cu in crostacei, sedimenti e acqua prelevati in siti della laguna di Lesina a diverso impatto antropico, al fine di verificare l'accumulo e la biomagnificazione nei diversi comparti. I sedimenti sono il comparto con concentrazioni di metalli più elevati rispetto alle specie ittiche esaminate, che a loro volta hanno mostrato per alcuni elementi concentrazioni differenti rispetto ai siti di campionamento. I risultati preliminari ci permettono di affermare che è possibile utilizzare Melicertus kerathurus come indicatore di inquinamento da metalli negli ambienti lagunari.

Published
2005

14. A selective ER-phagy exerts procollagen quality control via a Calnexin-FAM134B complex

Author

Forrester, Alison, De Leonibus, Chiara, Grumati, Paolo, Fasana, Elisa, Piemontese, Marilina, Staiano, Leopoldo, Fregno, Ilaria, Raimondi, Andrea, Marazza, Alessandro, Bruno, Gemma, Iavazzo, Maria, Intartaglia, Daniela, Seczynska, Marta, Van Anken, Eelco, Conte, Ivan, De Matteis, Maria Antonietta, Dikic, Ivan, Molinari, Maurizio, and Settembre, Carmine

Subjects
570 Life sciences, biology, 500 Science, 3. Good health
Abstract

Autophagy is a cytosolic quality control process that recognizes substrates through receptor-mediated mechanisms. Procollagens, the most abundant gene products in Metazoa, are synthesized in the endoplasmic reticulum (ER), and a fraction that fails to attain the native structure is cleared by autophagy. However, how autophagy selectively recognizes misfolded procollagens in the ER lumen is still unknown. We performed siRNA interference, CRISPR-Cas9 or knockout-mediated gene deletion of candidate autophagy and ER proteins in collagen producing cells. We found that the ER-resident lectin chaperone Calnexin (CANX) and the ER-phagy receptor FAM134B are required for autophagy-mediated quality control of endogenous procollagens. Mechanistically, CANX acts as co-receptor that recognizes ER luminal misfolded procollagens and interacts with the ER-phagy receptor FAM134B. In turn, FAM134B binds the autophagosome membrane-associated protein LC3 and delivers a portion of ER containing both CANX and procollagen to the lysosome for degradation. Thus, a crosstalk between the ER quality control machinery and the autophagy pathway selectively disposes of proteasome-resistant misfolded clients from the ER.

15. A selective ER-phagy exerts procollagen quality control via a Calnexin-FAM134B complex

Author

Forrester, Alison, De Leonibus, Chiara, Grumati, Paolo, Fasana, Elisa, Piemontese, Marilina, Staiano, Leopoldo, Fregno, Ilaria, Raimondi, Andrea, Marazza, Alessandro, Bruno, Gemma, Iavazzo, Maria, Intartaglia, Daniela, Seczynska, Marta, van Anken, Eelco, Conte, Ivan, Matteis, Maria Antonietta De, Dikic, Ivan, Molinari, Maurizio, and Settembre, Carmine

Subjects
collagen, autophagy, endoplasmic reticulum, Calnexin, FAM134B, 3. Good health
Abstract

Autophagy is a cytosolic quality control process that recognizes substrates through receptor‐mediated mechanisms. Procollagens, the most abundant gene products in Metazoa, are synthesized in the endoplasmic reticulum (ER), and a fraction that fails to attain the native structure is cleared by autophagy. However, how autophagy selectively recognizes misfolded procollagens in the ER lumen is still unknown. We performed siRNA interference, CRISPR‐Cas9 or knockout‐mediated gene deletion of candidate autophagy and ER proteins in collagen producing cells. We found that the ER‐resident lectin chaperone Calnexin (CANX) and the ER‐phagy receptor FAM134B are required for autophagy‐mediated quality control of endogenous procollagens. Mechanistically, CANX acts as co‐receptor that recognizes ER luminal misfolded procollagens and interacts with the ER‐phagy receptor FAM134B. In turn, FAM134B binds the autophagosome membrane‐associated protein LC3 and delivers a portion of ER containing both CANX and procollagen to the lysosome for degradation. Thus, a crosstalk between the ER quality control machinery and the autophagy pathway selectively disposes of proteasome‐resistant misfolded clients from the ER., The EMBO Journal, 38 (2), ISSN:0261-4189, ISSN:1460-2075

16. A selective ER‐phagy exerts procollagen quality control via a Calnexin‐FAM134B complex

Author

Forrester, Alison, Leonibus, Chiara De, Grumati, Paolo, Fasana, Elisa, Piemontese, Marilina, Staiano, Leopoldo, Fregno, Ilaria, Raimondi, Andrea, Marazza, Alessandro, Bruno, Gemma, Iavazzo, Maria, Intartaglia, Daniela, Seczynska, Marta, van Anken, Eelco, Conte, Ivan, De Matteis, Maria Antonietta, Dikic, Ivan, Molinari, Maurizio, Settembre, Carmine, Forrester, Alison, Leonibus, Chiara De, Grumati, Paolo, Fasana, Elisa, Piemontese, Marilina, Staiano, Leopoldo, Fregno, Ilaria, Raimondi, Andrea, Marazza, Alessandro, Bruno, Gemma, Iavazzo, Maria, Intartaglia, Daniela, Seczynska, Marta, van Anken, Eelco, Conte, Ivan, De Matteis, Maria Antonietta, Dikic, Ivan, Molinari, Maurizio, and Settembre, Carmine

Abstract

Autophagy is a cytosolic quality control process that recognizes substrates through receptor‐mediated mechanisms. Procollagens, the most abundant gene products in Metazoa, are synthesized in the endoplasmic reticulum (ER), and a fraction that fails to attain the native structure is cleared by autophagy. However, how autophagy selectively recognizes misfolded procollagens in the ER lumen is still unknown. We performed siRNA interference, CRISPR‐Cas9 or knockout‐mediated gene deletion of candidate autophagy and ER proteins in collagen producing cells. We found that the ER‐resident lectin chaperone Calnexin (CANX) and the ER‐phagy receptor FAM134B are required for autophagy‐mediated quality control of endogenous procollagens. Mechanistically, CANX acts as co‐receptor that recognizes ER luminal misfolded procollagens and interacts with the ER‐phagy receptor FAM134B. In turn, FAM134B binds the autophagosome membrane‐associated protein LC3 and delivers a portion of ER containing both CANX and procollagen to the lysosome for degradation. Thus, a crosstalk between the ER quality control machinery and the autophagy pathway selectively disposes of proteasome‐resistant misfolded clients from the ER.

17. Current methods to analyze lysosome morphology, positioning, motility and function

Author

Duarte C. Barral, Leopoldo Staiano, Cláudia Guimas Almeida, Dan F. Cutler, Emily R. Eden, Clare E. Futter, Antony Galione, André R. A. Marques, Diego Luis Medina, Gennaro Napolitano, Carmine Settembre, Otília V. Vieira, Johannes M. F. G. Aerts, Peace Atakpa‐Adaji, Gemma Bruno, Antonella Capuozzo, Elvira De Leonibus, Chiara Di Malta, Cristina Escrevente, Alessandra Esposito, Paolo Grumati, Michael J. Hall, Rita O. Teodoro, Susana S. Lopes, J. Paul Luzio, Jlenia Monfregola, Sandro Montefusco, Frances M. Platt, Roman Polishchuck, Maria De Risi, Irene Sambri, Chiara Soldati, Miguel C. Seabra, Barral, Duarte C [0000-0001-8867-2407], Staiano, Leopoldo [0000-0001-7017-1516], Guimas Almeida, Cláudia [0000-0001-9384-2896], Eden, Emily R [0000-0001-9352-5532], Marques, André RA [0000-0001-9674-3017], Vieira, Otília V [0000-0003-4924-1780], Escrevente, Cristina [0000-0002-2183-3947], Hall, Michael J [0000-0002-1579-1488], Teodoro, Rita O [0000-0002-0600-8842], Lopes, Susana S [0000-0002-6733-6356], Luzio, J Paul [0000-0003-3912-9760], Platt, Frances M [0000-0001-7614-0403], Polishchuck, Roman [0000-0002-7698-1955], Sambri, Irene [0000-0003-3500-6958], Seabra, Miguel C [0000-0002-6404-4892], Apollo - University of Cambridge Repository, Barral, Duarte C, Staiano, Leopoldo, Almeida, Cláudia Guima, Cutler, Dan F, Eden, Emily R, Futter, Clare E, Galione, Antony, Marques, André R A, Medina, Diego Lui, Napolitano, Gennaro, Settembre, Carmine, Vieira, Otília V, Aerts, Johannes M F G, Atakpa-Adaji, Peace, Bruno, Gemma, Capuozzo, Antonella, De Leonibus, Elvira, Di Malta, Chiara, Escrevente, Cristina, Esposito, Alessandra, Grumati, Paolo, Hall, Michael J, Teodoro, Rita O, Lopes, Susana S, Luzio, J Paul, Monfregola, Jlenia, Montefusco, Sandro, Platt, Frances M, Polishuck, Roman, De Risi, Maria, Sambri, Irene, Soldati, Chiara, and Seabra, Miguel C

Subjects
Membrane contact site, TFEB, Lysosome exocytosi, lysosome biogenesis, endolysosomes, membrane contact sites, Lysosomal storage disease, Cell Biology, Lysosome-related organelle, Lysosome, Biochemistry, Endolysosome, lysosome-related organelles, lysosomes, Structural Biology, lysosome exocytosis, Genetics, mTOR, Lysosome biogenesi, lysosomal storage diseases, Molecular Biology, Metabolic Networks and Pathways, Signal Transduction
Abstract

Funder: Maratona da Saúde, Funder: Royal Society Wolfson, Funder: Wellcome; Id: http://dx.doi.org/10.13039/100010269, Since the discovery of lysosomes more than 70 years ago, much has been learned about the functions of these organelles. Lysosomes were regarded as exclusively degradative organelles, but more recent research has shown that they play essential roles in several other cellular functions, such as nutrient sensing, intracellular signalling and metabolism. Methodological advances played a key part in generating our current knowledge about the biology of this multifaceted organelle. In this review, we cover current methods used to analyze lysosome morphology, positioning, motility and function. We highlight the principles behind these methods, the methodological strategies and their advantages and limitations. To extract accurate information and avoid misinterpretations, we discuss the best strategies to identify lysosomes and assess their characteristics and functions. With this review, we aim to stimulate an increase in the quantity and quality of research on lysosomes and further ground-breaking discoveries on an organelle that continues to surprise and excite cell biologists.

Published
2022

18. A selective ER ‐phagy exerts procollagen quality control via a Calnexin‐ FAM 134B complex

Author

Alison Forrester, Alessandro Marazza, Elisa Fasana, Ivan Dikic, Leopoldo Staiano, Marilina Piemontese, Maria Iavazzo, Carmine Settembre, Gemma Bruno, Chiara De Leonibus, Daniela Intartaglia, Ilaria Fregno, Maria Antonietta De Matteis, Ivan Conte, Marta Seczynska, Paolo Grumati, Maurizio Molinari, Eelco van Anken, Andrea Raimondi, Forrester, A, De Leonibus, C, Grumati, P, Fasana, E, Piemontese, M, Staiano, L, Fregno, I, Raimondi, A, Marazza, A, Bruno, G, Iavazzo, M, Intartaglia, D, Seczynska, M, van Anken, E, Conte, I, De Matteis, Ma, Dikic, I, Molinari, M, Settembre, C, Forrester, Alison, De Leonibus, Chiara, Grumati, Paolo, Fasana, Elisa, Piemontese, Marilina, Staiano, Leopoldo, Fregno, Ilaria, Raimondi, Andrea, Marazza, Alessandro, Bruno, Gemma, Iavazzo, Maria, Intartaglia, Daniela, Seczynska, Marta, van Anken, Eelco, Conte, Ivan, DE MATTEIS, Maria Antonietta, Dikic, Ivan, Molinari, Maurizio, and Settembre, Carmine

Subjects
collagen, Autophagosome, Protein Folding, autophagy, Calnexin, Oryzias, Biology, Article, General Biochemistry, Genetics and Molecular Biology, Cell Line, Mice, 03 medical and health sciences, 0302 clinical medicine, Lysosome, medicine, Animals, Humans, ddc:610, Membrane & Intracellular Transport, Receptor, Molecular Biology, 030304 developmental biology, 0303 health sciences, General Immunology and Microbiology, endoplasmic reticulum, FAM134B, General Neuroscience, Endoplasmic reticulum, Autophagy, Intracellular Signaling Peptides and Proteins, Membrane Proteins, Articles, 500 Science, 3. Good health, Cell biology, Crosstalk (biology), medicine.anatomical_structure, Gene Knockdown Techniques, Chaperone (protein), biology.protein, 570 Life sciences, biology, Autophagy & Cell Death, Microtubule-Associated Proteins, Procollagen, 030217 neurology & neurosurgery, HeLa Cells
Abstract

Autophagy is a cytosolic quality control process that recognizes substrates through receptor-mediated mechanisms. Procollagens, the most abundant gene products in Metazoa, are synthesized in the endoplasmic reticulum (ER), and a fraction that fails to attain the native structure is cleared by autophagy. However, how autophagy selectively recognizes misfolded procollagens in the ER lumen is still unknown. We performed siRNA interference, CRISPR-Cas9 or knockout-mediated gene deletion of candidate autophagy and ER proteins in collagen producing cells. We found that the ER-resident lectin chaperone Calnexin (CANX) and the ER-phagy receptor FAM134B are required for autophagy-mediated quality control of endogenous procollagens. Mechanistically, CANX acts as co-receptor that recognizes ER luminal misfolded procollagens and interacts with the ER-phagy receptor FAM134B. In turn, FAM134B binds the autophagosome membrane-associated protein LC3 and delivers a portion of ER containing both CANX and procollagen to the lysosome for degradation. Thus, a crosstalk between the ER quality control machinery and the autophagy pathway selectively disposes of proteasome-resistant misfolded clients from the ER.

Published
2018
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19. Thiirancarboxamides as inhibitors of papain.

Author

Bruno G and Schirmeister T

Subjects
Carboxylic Acids chemistry, Carboxylic Acids pharmacology, Enzyme Inhibitors chemistry, Enzyme Inhibitors pharmacology, Structure-Activity Relationship, Carboxylic Acids chemical synthesis, Enzyme Inhibitors chemical synthesis, Papain antagonists & inhibitors
Abstract

Derivatives of the thiirancarboxylic acid building-block containing a peptide bond were synthesised and screened against the model cysteine protease papain. The most active of the series showed a second-order rate constant of inactivation comparable to that of the parent compound. The insertion of a peptide moiety seems to compensate the lack of a free carboxylate interacting with the histidinium ion at the enzyme's active site.

Published
2004
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