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Human islet mass,morphology, and survival after cryopreservation using the Edmonton protocol
Authors:Priya M Miranda  Viswanathan Mohan  Sekhar Ganthimathy  Ranjit M Anjana  S Gunasekaran  Venkatachalam Thiagarajan  Thomas A Churchill  Tatsuya Kin  AM James Shapiro  Jonathan RT Lakey
Institution:1.Madras Diabetes Research Foundation & Dr. Mohan’s Diabetes Specialties Centre; WHO Collaborating Centre for Noncommunicable Diseases-Prevention and Control; Chennai, Tamilnadu, India;2.Saveetha Medical College; Thandalam, Chennai, India;3.Christian Medical College; Vellore, Tamil Nadu, India;4.Tamilnadu Veterinary and Animal Science University; Chennai, India;5.University of Alberta; Edmonton, Alberta, Canada;6.University of California; Irvine, CA USA
Abstract:The aim of this study was to assess recovery, cell death, and cell composition of post-thaw cultured human islets. Cryopreserved islets were provided by the Clinical Islet Transplant Program, Edmonton, Canada. Islets were processed using media prepared in accordance with Pre-Edmonton and Edmonton protocols. Cryopreserved islets were rapidly thawed and cultured for 24 h, 3 d, 5 d, and 7 d, following which they were processed for histology. Islet quantification, integrity, morphology and tissue turnover were studied via hematoxylin and eosin stained sections. Ultrastructure was studied by electron microscopy and endocrine cell composition by immunohistochemistry. Using the Pre-Edmonton protocol, islet recovery was 50.1% and islet survival was 50% at 24 h while for the Edmonton protocol, the islet recovery was 69.4% (p < 0.001) and islet survival, 50% at ≈2.5 d. With an increasing culture duration although the physical integrity was retained there was an increasing loss of cohesivity both at light microscopic and at ultrastructure level regardless of the protocols used. Percentage islet survival and tissue turnover correlated negatively with culture duration in both protocols. The Edmonton protocol appears to preserve the islets better. However, culture duration adversely affects islet survival and quality, indicating the need for more optimal cryopreservation and culture techniques.
Keywords:islet transplantation  cryopreservation  post-thaw culture  islet isolation  clinical phase  pre-clinical phase  ultrastructure TUNEL  immunohistochemistry
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