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Background: Differential diagnosis between complete hydatidiform mole, partial hydatidiform mole and hydropic abortion, known as hydropic placentas is still a challenge for pathologists but it is very important for patient management. Objective: We analyzed the nuclear DNA content of various types of hydropic placentas by flowcytometry. Materials and Methods: DNA ploidy analysis was performed in 20 non-molar [hydropic and non-hydropic spontaneous aboltions] and 20 molar [complete and partial moles], formalin-fixed, paraffin-embedded tissue samples by flow cytometry. The criteria for selection were based on the histopathologic diagnosis. Results: Of 10 cases histologically diagnosed as complete hydatiform mole, 9 cases yielded diploid histograms, and 1 case was tetraploid. Of 10 partial hydatidiform moles, 8 were triploid and 2 were diploid. All of 20 cases diagnosed as spontaneous abortions [hydropic and non-hydropic] yielded diploid histograms. Conclusion: These findings signify the importance of the combined use of conventional histology and ploidy analysis in the differential diagnosis of complete hydatidiform mole, partial hydatidiform mole and hydropic abortion
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Multiple sclerosis [MS] is the most common inflammatory disease of the CNS. Experimental autoimmune encephalomyelitis [EAE] is a widely used model for MS. In the present research, our aim was to test the therapeutic efficacy of Calcium [Ca] in an experimental model of MS. In this study the experiment was done on C57BL/6 mice. EAE was induced using 200 micro g of the MOG[35-55] peptide emulsified in CFA and injected subcutaneously on day 0 over two flank areas. In addition, 250 ng of pertussis toxin was injected on days 0 and 2. In the treatment group, 30 mg/kg Ca was administered intraperitoneally four times at regular 48 hour intervals. The mice were sacrificed 21 days after EAE induction and blood samples were taken from their hearts. The brains of mice were removed for histological analysis and their isolated splenocytes were cultured. Our results showed that treatment with Ca caused a significant reduction in the severity of the EAE. Histological analysis indicated that there was no plaque in brain sections of Ca treated group of mice whereas 4 +/- 1 plaques were detected in brain sections of controls. The density of mononuclear infiltration in the CNS of Ca treated mice was lower than in controls. The serum level of Nitric Oxide in the treatment group was lower than in the control group but was not significant. Moreover, the levels of IFN- gamma in cell culture supernatant of splenocytes in treated mice were significantly lower than in the control group. The data indicates that Ca intervention can effectively attenuate EAE progression
Assuntos
Animais de Laboratório , Cálcio , Encefalomielite Autoimune Experimental , Camundongos , Óxido Nítrico , Sistema Nervoso CentralRESUMO
Today, the intractions of the immune system of the immune system, nutrition, and nervous system are one of the main research areas of interest in immunology and disease treatment. Due to changes in the mood, behavior, and diet of an individual during fasting period, the body's internal homeostasis is affected. The aim of the present study was to evaluate the effects of Ramadan fasting on lymphocyte subgroups, which are the main specific immune cells in the body. For this purpose, in years 1999 and 2000, thirty?eight healthy Muslims [9 females and 29 males], within the age range of 17 to 51 years [mean age=35.4 years], were assessed before the start and one day before the end of Ramadan. The pre-Lymphocytic subpopulations analysis was conducted using flow cytometery. The results showed that the percentage of total lymphocytes was 25.82% and 26.23% in the pre- and late- Ramadan periods, respectively; the observed difference was insignificant. However, the absolute lymphocyte counts were 2.3x103 and 2.1x103 mm3 before and late Ramadan, respectively, and the difference was considered significant [P-value=0.06]. The percentage of CD3+ cells [T cells] was 70.12% before Ramadan and 70.25% late Ramadan, and the absolute lymphocyte counts were 1.6x103 and 1.5x103 mm3, respectively; therefore, the differences were not significant. Regarding the subgroups of CD4+cells [TH], the percentage ratios of the cells were 53.46% and 52.8% in the pre- and late Ramadan periods, and the absolute counts were 0.087x103 and 0.081x103 mm3, respectively; however, the differences were not significant in this cell subgroup. The percentage of CD8+ [TC] cells was 37.7% before Ramadan and 37.8% late Ramadan, and the absolute counts were 0.6x103 and 0.54x103 mm3 in the pre- and late-Ramadan periods, respectively; therefore, the differences were considered insignificant. In addition, the percentage ratios of Blymphocytes cells were 14.56% and 14.74% in the pre- and late-Ramadan periods, and the absolute count changed from 0.35x103 to 0.3x103 mm3. According to the results, the differences were not significant, therefore, it seems Ramadan fasting does not affect these cells. Moreover, the percentage of activated T cells or TDR+, which are involved in specific immune responses, has not been affected by fasting. In fact, the percentage ratios were reported as 11.14% and 10.54% in the pre- and late-Ramadan periods, and the absolute count changed from 0.14x103 to 0.11x103 mm3; the differences were not considered significant. Finally, the ratio of CD4+/CD8+ cells or TH/TC changed from 1.48% before Ramadan to 1.5% late this month; however, this difference was insignificant. Thus, the overall results indicate that Ramadan fasting during winter does not affect the lymphocyte count, percentage ratio, and the main lymphocyte subpopulations
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Recent studies on human indicate that the introduction of therapeutic use of tolerogenic dendritic cell [DC] for chronic inflammatory conditions is imminent. For the purpose of defining CGRP potency in tolerogenic DC production, we investigated the phenotype and IL-12 production of DCs generated from the monocytes of rheumatoid arthritis [RA] patients in the presence of the calcitonin gene-related peptide [CDRP], as a multifunctional neuropeptide. DCs were generated from isolated monocytes from four resistant and two early female RA patients using IL-4, GM-CSF, and CGRP at concentrations of 0, 1, and 100 nM. Then, the phenotype of neuropeptide-treated or untreated DCs was determined using flow cytometry and the IL-12 production was measured by ELISA. Our study showed that, on the last day of the culture, at a concentration of 1 nM CGRP, the mean fluorescence intensity [MFI] for CD80 increased [14.13%] and the MFIs for CD83, CD86, and HLA-DR decreased [14.57%, 5.28%, and 6.88% respectively]. Moreover, at 100 nM CGRP concentration, the MFI for CD80 increased [11.10%] and the MFIs for CD83, CD86, and HLA-DR decreased [4.27%, 18.60%, and 19.75% respectively]. In addition, our results indicated that the mean concentrations of IL-12 produced at 0, 1, and 100 nm CGRP concentrations measured 13.72 +/- 2.41, 11.01 +/- 1.61, and 7 +/- 1.34 pg/ml respectively. Decreased CD83, CD86, and HLA-DR expression and reduced IL-12 production by CGRP were found in the RA patients' monocyte-derived DCs. CD83 is a well-defined DC activation marker. HLA-DR and CD86 are appropriate molecules for inducing an immune response. IL-12 promotes cell-mediated immunity. Therefore we suggest that CGRP may be used as an inducer in the production of tolerogenic DCs
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Systemic Lupus Eyrythematosus [SLE] is an autoimmune disease characterized by antibodies to nuclear antigens, particularly anti-dsDNA. Imbalance between production and destruction of immune cells causes cytopenia. Sex hormones have im-munomodulatory effects; estrogen increases the production of autoantibodies in SLE prone NZB/NZW mice. To investigate the relationship between sex hormones, anti-dsDNA, and lymphocyte subsets in Iranian patients with SLE. 38 SLE patients [28 females and 10 males] meeting 4 of 11 ACR revised criteria for SLE classification, and 20 age and sex matched healthy individuals [10 females and 10 males] participated in this study. Lymphocyte subsets were analyzed using flow cy-tometric analysis. Serum anti-dsDNA levels and sex hormones concentrations were determined using commercial ELISA and RIA kits, respectively. The absolute count of white blood cells, lymphocytes, T lymphocytes [CD3[+], T helper cells [CD3[+]CD4[+], B cells [CD19[+] and Nk cells [CD3[-] CD16[+]CD56[+] in SLE patients diminished significantly in comparison to control group [p<0.05]. IgG anti-dsDNA antibody levels were significantly higher in patients compared to controls as expected [p<0.05]. Prolactin increased significantly, while DHEAS showed a significant decrease in SLE patients compared with the controls [p<0.05], however the level of estrogen did not have any significant difference in SLE patients in comparison to controls. Increased concentration of prolactin together with a simultaneous decrease in serum DHEAS in SLE patients are associated with anti-dsDNA elevation and a decrease in almost all lymphocyte subsets