We aimed to study the expression of Pgp on CD4+IFN-ϒ+ Th1, CD4+IL

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We aimed to study the expression of Pgp on CD4+IFN-ϒ+ Th1, CD4+IL-4+ Th2 and CD4+CD25+FoxP3+ regulatory T lymphocyte (Treg) with their imbalance in steroid response in NS. Methods: From patients of NS, 22 patients in sustained remission, 24 in relapse, and 21 steroid resistant patients and 14 healthy controls were included in the study .Circulating Treg, Th1 and Th2 lymphocytes and P-gp Expression

on these T reg, Th1 and Th2 lymphocytes in patients in sustained remission, relapse, steroid resistant (SRNS) and healthy control were measured. this website Results: The absolute expression of Pgp was greater in relapsed (83.51 ± 37.22, P = 0.001) and SRNS (101.72 ± 44.91, P = 0.001) compared to that of patients in remission (33.16 ± 23.97) and controls (33.38 ± 17.05) Table1. The % of Th1 cells was significantly lesser in patients with sustained remission (10.37 ± 3.49) compared to that of patients during relapse (16.18 ± 7.19; P = 0.008); SRNS patients (20.24 ± 7.01; P = 0.001); and in controls (18.38 ± 3.28;

P = 0.006) Fig 1A. Th2 cells (%) in patients with remission (5.18 ± 3.12) was significantly less than that of relapsed (9.89 ± 5.23; P = 0.006) or SRNS patients (10.74 ± 5.91; P = 0.001); and similar to that of control subjects (4.91 ± 1.24) p = 1.0. Fig 1B. The Treg cells were significantly higher in controls and remission compared Trichostatin A in vitro to that PLEKHB2 of SRNS and relapsed patients. Fig1C. The

ratio of Th1/ Tregs, Th2/Tregs and Th1/ Th2 are shown in Figure 1D,E,F indicate that imbalance between Treg and Teff is responsible for remission and SRNS state. Conclusion: The imbalance of Treg and Teff cells with expression of P-gp plays role in steroid response in NS. SHIOHIRA SHUNJI1, YOSHIDA TAKUMI1,2, SUGIURA HIDEKAZU1, NISHIDA MIKI1, NITTA KOSAKU1, TSUCHIYA KEN1 1Department of Medicine IV, Tokyo Women’s Medical University; 2Yoshida Medical Clinic Introduction: Sphingosine 1-phosphate (S1P), a bioactive lipid mediator, has been suggested to be involved in the mechanism of renal fibrosis. Previously, we have shown the direct effects of S1P on the fibrotic process in the unilateral ureteral obstruction (UUO) model using nude mice which were characterized by deficit of immune response. To get more insight into roles for S1P and receptor subtype effects in vitro, we performed using antagoists and siRNAs knockdown of receptor subtypes. Methods: Normal rat kidney interstitial fibroblast (NRK-49F) cells were stimulated with exogenous S1P and the expressions (mRNA/Western blotting) of a-SMA, E-cadherin, collagen type 1 (COL1), collagen type 4 (COL4), tissue inhibitor of matrix metalloproteinase-1 (TIMP1) and plasminogen activator inhibitor-1 (PAI1) were examined. To specify the kidney specific signal pathway, antagonists and siRNAs targeted to S1P receptor subtypes were generated.

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