5A), microvillar
extensions (Fig. 5C) and, for SEMA6A only, motility in T cells (Fig. 6A). Interestingly, SEMA-mediated cytoskeletal interference did not affect the overall β1-integrin-stimulated front-rear polarization or receptor-segregation (Fig. 5B and C) thereby essentially differing from actin cytoskeletal https://www.selleckchem.com/products/abc294640.html paralysis induced on MV exposure of these cells 18, 47. In line with hypothesis, induction of ceramides as found relevant for MV actin interference 18 was not detectable on SEMA3A/6A exposure of T cells (not shown) indicating the SEMA-induced signalling may not involve SMase activation. In addition to adding to the current view on the role and regulation of human SEMA receptors in the IS in general (such as plexA1 IS recruitment and its importance for IS function in T cells, plexA4 expression in human T cells, plexA1/NP-1 turnover in maturing DC, SEMA3A and SEMA6A in regulation of T-cell protrusions and chemokinetic migration), our study to the best of our knowledge is the first to address regulation of those by a pathogen and their importance in the established MV interference with IS function. Recruitment to and concentration of SEMA receptors
to the IS might, however, also be of relevance for viral transmission there as indicated by the function of NP-1 as physical and functional partners of HTLV env proteins during transmission in the virological synapse 32, 52. Primary human cells were obtained from the Department of Transfusion Medicine, University of Würzburg, Tamoxifen and analyzed anonymized. All experiments involving human material were conducted according to the principles expressed in the Declaration of Helsinki and ethically approved by the Ethical Committee of the Medical Faculty of the University of Würzburg. Primary human T cells were enriched from peripheral blood
obtained from healthy Aldehyde dehydrogenase donors by Ficoll gradient centrifugation followed on nylon wool columns and maintained in RPMI1640/10% FBS. Immature DC (iDC) were generated from monocytes in RPMI 1640/5% FBS by culture with GM-CSF (500 U/mL; Strathmann) and 250 U/mL IL-4 (250 U/mL; Promocell) and, when indicated, exposed to LPS (100 ng/mL) (LPS-DC) or a mock preparation obtained by freeze/thawing and subsequent low-speed centrifugation of human lymphoblastoid BJAB cells (kept in RPMI1640/10% FBS)(mock-DC) for 24 h. The MV WT strain WTF and the MVrecombinant MGV (expressing VSV-G protein instead of the MV gps 53) were grown on human lymphoblastoid BJAB cells and titrated on marmoset lymphoblastoid B95a cells (kept in RPMI1640/10% FBS). For exposure experiments, MV was purified by sucrose gradient ultracentrifugation as was the mock control from uninfected BJAB cells. T cells were co-cultured with MV (at a multiplicity of infection (m.o.i.) of 0.