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Showing 2 results for Nabiuni

Maryam Kakaei, Zahra Nazari, Latifeh Karimzadeh, M Nabiuni,
Volume 13, Issue 1 (5-2013)
Abstract

The in-vitro culture of  immature ovarian follicles is used to examine the factors that regulate follicle development and may ultimately provide options  for  reproductive  infertility. Normal follicular development of an oocyte that is capable of fertilization and embryonic development depends upon a complex sequence of cellular interactions within the follicle . Honey Bee Venom (HBV) contains some biological active components which has been demonstrated it,s promoting effect on ovulation up to 70 % in rats . The aim of this research is study of the effect of HBV on in-vitro maturation of different type of preantral follicles. In this research, unmature follicles were taken from 14 day-old mice and cultured in &alpha-minimal essential medium (&alpha-MEM) and divided to small, medium and large preantral follicles and treated with 1µg/ml BV. Then diameter of follicle was measured until 4th days. Finally, morphological appearance of mature oocytes was studied. Studies of follicle diameters and flowcytometry showed HBV led to an increase in follicle diameters (p<0.001). Amount of GV was 53 %(control group) and 31.4 (treatment group)that was significative (p<0.001). Developing up to meiosis I was 30% (control group) and 43.2% (treatment group) and developing up to meiosis II was 15% (control) and 22.3% (treatment group). In brief, we are confirmed that honey bee venom has led to significant changes in in-vitro maturation of preantral follicles and consequently, better performance for fertilization.
E Hoveazi, M Nabiuni, K Parivar, M Masomi, J Agh,
Volume 15, Issue 1 (4-2015)
Abstract

Today, induced pluripotent cells (iPS) have been recognized as a new and good cell source for cell therapy. In this study, we examined whether human iPS cells, cultured on scaffolds, can differentiate into definitive endodermal cells, as precursor for hepatocytes, pancreatic and lung cells. Embryoid bodies (EBs) composed of iPS cells then EBs were seeded on electrospinning nanofiber scaffold (PCL). The cells were differentiated into definitive endoderm by using IDE1(induced definitive endoderm). Expression of definitive endoderm markers including Sox17, FoxA2 and Gsc were confirmed by Immunocytochemistry attaining and RT-PCR analysis. In the present study, cells morphology and cells viability were evaluated by using a scanning electron microscopy and MTT assay respectively.The results of this study demonstrated the positive effect of 3D cultures, by using suitable factors, on definitive endoderm differentiation.definitive endoderm by using IDE1(induced definitive endoderm). Expression of definitive endoderm markers including Sox17, FoxA2 and Gsc were confirmed by Immunocytochemistry attaining and RT-PCR analysis. In the present study, cells morphology and cells viability were evaluated by using a scanning electron microscopy and MTT assay respectively.The results of this study demonstrated the positive effect of 3D cultures, by using suitable factors, on definitive endoderm differentiation.

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