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Ex-vivo modeling of leukemic stem cell niche : Sub - classifying CD34⁺ population according to quiescence / Nesreen Hamdi Mahmoud ; Supervised Iman Ahmed Maher Mansour , Nadia Ibrahim Sewilam

بواسطة: المساهم: نوع المادة : نصاللغة: الإنجليزية تفاصيل النشر: Cairo : Nesreen Hamdi Mahmoud , 2014الوصف: 145 P. : charts , facsimiles ; 25cmعنوان آخر:
  • علي حسب درجة سكونها CD 34⁺التمثيل الخارجي للبيئة المحيطة بالخلايا الجذعية في حالات اللوكيميا الحادة لتقسيم الخلايا الجذعية اللوكيميا الحادة [عنوان مضاف عنوان الصفحة]
الموضوع: موارد على الإنترنت: Available additional physical forms:
  • Issued also as CD
ملاحظة الأطروحة: Thesis (Ph.D.) - Cairo University - Faculty of Medicine - Department of Clinical and Chemical Pathology ملخص: Acute myeloid leukemia is a paradigm of cancer stem (or leukemia initiating) cells. Stem cell niche acts as a sanctuary for the stem cells that allow their survival, self-renewal and regulated proliferation. In parallel with leukemogenic events in the hematopoietic system, the niche is converted into an environment with dominant signals that favor cell proliferation and growth. Using ex-vivo culture, the present study simulated the bone marrow niche. Mononuclear cells from bone marrow aspirates of AML cases and controls were co-cultured on confluent mesenchymal stem cell layer. We estimated the percent of cells in G0 phase of the cell cycle and percentage of CD34⁺38- cells in the 3 layers of the ex-vivo culture. In AML cases, the distribution of the CD34⁺38- cells, revealed a significant difference between the 3 layers (p < 0.001), with a significantly lower percent in layer 3. A statistically significant difference between layer 3 of the cases and of the controls (p < 0.026), was also detected. No statistically significant difference in mean percentage of quiescent cells (PI⁺ Ki-67- ) was found on comparing the percentage of G0 cells in layer 1 and 2 of cases to those of control subjects. It was concluded that mesenchymal cell interaction with leukemic cells resulted in an altered distribution of the CD34⁺38- cell compartment when compared to normal but did not affect the cycling status of the cells
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المقتنيات
نوع المادة المكتبة الحالية المكتبة الرئيسية رقم الاستدعاء رقم النسخة حالة الباركود
Thesis قاعة الرسائل الجامعية - الدور الاول المكتبة المركزبة الجديدة - جامعة القاهرة Cai01.11.07.Ph.D.2014.Ne.E (استعراض الرف(يفتح أدناه)) لا تعار 01010110065115000
CD - Rom مخـــزن الرســائل الجـــامعية - البدروم المكتبة المركزبة الجديدة - جامعة القاهرة Cai01.11.07.Ph.D.2014.Ne.E (استعراض الرف(يفتح أدناه)) 65115.CD لا تعار 01020110065115000

Thesis (Ph.D.) - Cairo University - Faculty of Medicine - Department of Clinical and Chemical Pathology

Acute myeloid leukemia is a paradigm of cancer stem (or leukemia initiating) cells. Stem cell niche acts as a sanctuary for the stem cells that allow their survival, self-renewal and regulated proliferation. In parallel with leukemogenic events in the hematopoietic system, the niche is converted into an environment with dominant signals that favor cell proliferation and growth. Using ex-vivo culture, the present study simulated the bone marrow niche. Mononuclear cells from bone marrow aspirates of AML cases and controls were co-cultured on confluent mesenchymal stem cell layer. We estimated the percent of cells in G0 phase of the cell cycle and percentage of CD34⁺38- cells in the 3 layers of the ex-vivo culture. In AML cases, the distribution of the CD34⁺38- cells, revealed a significant difference between the 3 layers (p < 0.001), with a significantly lower percent in layer 3. A statistically significant difference between layer 3 of the cases and of the controls (p < 0.026), was also detected. No statistically significant difference in mean percentage of quiescent cells (PI⁺ Ki-67- ) was found on comparing the percentage of G0 cells in layer 1 and 2 of cases to those of control subjects. It was concluded that mesenchymal cell interaction with leukemic cells resulted in an altered distribution of the CD34⁺38- cell compartment when compared to normal but did not affect the cycling status of the cells

Issued also as CD

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