Your search keyword '"Zamoyska R"' showing total 2 results

1. miR-181a/b-1 controls thymic selection of Treg cells and tunes their suppressive capacity

Author

Bhandoola, A, Lyszkiewicz, M, Winter, SJ, Witzlau, K, Foehse, L, Brownlie, R, Puchalka, J, Verheyden, NA, Kunze-Schumacher, H, Imelmann, E, Blume, J, Raha, S, Sekiya, T, Yoshimura, A, Frueh, JT, Ullrich, E, Huehn, J, Weiss, S, Gutierrez, MG, Prinz, I, Zamoyska, R, Zietara, N, Krueger, A, Bhandoola, A, Lyszkiewicz, M, Winter, SJ, Witzlau, K, Foehse, L, Brownlie, R, Puchalka, J, Verheyden, NA, Kunze-Schumacher, H, Imelmann, E, Blume, J, Raha, S, Sekiya, T, Yoshimura, A, Frueh, JT, Ullrich, E, Huehn, J, Weiss, S, Gutierrez, MG, Prinz, I, Zamoyska, R, Zietara, N, and Krueger, A

Abstract

The interdependence of selective cues during development of regulatory T cells (Treg cells) in the thymus and their suppressive function remains incompletely understood. Here, we analyzed this interdependence by taking advantage of highly dynamic changes in expression of microRNA 181 family members miR-181a-1 and miR-181b-1 (miR-181a/b-1) during late T-cell development with very high levels of expression during thymocyte selection, followed by massive down-regulation in the periphery. Loss of miR-181a/b-1 resulted in inefficient de novo generation of Treg cells in the thymus but simultaneously permitted homeostatic expansion in the periphery in the absence of competition. Modulation of T-cell receptor (TCR) signal strength in vivo indicated that miR-181a/b-1 controlled Treg-cell formation via establishing adequate signaling thresholds. Unexpectedly, miR-181a/b-1-deficient Treg cells displayed elevated suppressive capacity in vivo, in line with elevated levels of cytotoxic T-lymphocyte-associated 4 (CTLA-4) protein, but not mRNA, in thymic and peripheral Treg cells. Therefore, we propose that intrathymic miR-181a/b-1 controls development of Treg cells and imposes a developmental legacy on their peripheral function.

Published

2019

2. Centrosome docking at the immunological synapse is controlled by Lck signaling

Author

Tsun, A, Qureshi, I, Stinchcombe, JC, Jenkins, MR, de la Roche, M, Kleczkowska, J, Zamoyska, R, Griffiths, GM, Tsun, A, Qureshi, I, Stinchcombe, JC, Jenkins, MR, de la Roche, M, Kleczkowska, J, Zamoyska, R, and Griffiths, GM

Abstract

Docking of the centrosome at the plasma membrane directs lytic granules to the immunological synapse. To identify signals controlling centrosome docking at the synapse, we have studied cytotoxic T lymphocytes (CTLs) in which expression of the T cell receptor-activated tyrosine kinase Lck is ablated. In the absence of Lck, the centrosome is able to translocate around the nucleus toward the immunological synapse but is unable to dock at the plasma membrane. Lytic granules fail to polarize and release their contents, and target cells are not killed. In CTLs deficient in both Lck and the related tyrosine kinase Fyn, centrosome translocation is impaired, and the centrosome remains on the distal side of the nucleus relative to the synapse. These results show that repositioning of the centrosome in CTLs involves at least two distinct steps, with Lck signaling required for the centrosome to dock at the plasma membrane.

Published

2011