中国组织工程研究与临床康复
中國組織工程研究與臨床康複
중국조직공정연구여림상강복
JOURNAL OF CLINICAL REHABILITATIVE TISSUE ENGINEERING RESEARCH
2010年
18期
3301-3304
,共4页
王艳盛%谢莎莎%王燕蓉%黑长春%郑小敏
王豔盛%謝莎莎%王燕蓉%黑長春%鄭小敏
왕염성%사사사%왕연용%흑장춘%정소민
绵羊卵巢%异种移植%玻璃化冻存%促卵泡刺激素%组织移植
綿羊卵巢%異種移植%玻璃化凍存%促卵泡刺激素%組織移植
면양란소%이충이식%파리화동존%촉란포자격소%조직이식
背景:卵巢皮质片移植是无血管吻合移植,因此,提高卵巢组织对冻存-解冻和移植后缺血的耐受力是提高冻存后移植物卵泡存活和延长功能寿命的关键环节.目的:观察促卵泡刺激素在玻璃化冻存过程中对绵羊卵巢组织形态和功能的保存效果,为成人卵巢组织的冻存提供技术方法.方法:BALB/c品系雌性裸鼠随机分为3组.均行羊卵巢皮质片裸鼠异位移植:①新鲜移植对照组,取材后即移植.②玻璃化冻存移植组,采用玻璃化冻存解冻后移植,所用液体均未添加促卵泡刺激素.③添加促卵泡刺激素的玻璃化冻存移植组,采用冷冻液、解冻液和培养液均添加促卵泡刺激素的玻璃化冻存后移植.移植后检测受体鼠动情周期恢复率、恢复时间、卵泡数和发育状况,于移植后4周取移植卵巢进行组织学观察、并行血清雌二醇水平分析.结果与结论:含促卵泡刺激素的玻璃化冻存移植组与新鲜移植组相比动情周期恢复率、每高倍视野卵泡计数差异均无显著性意义(P>0.05),卵泡计数高于未添加促卵泡刺激素的玻璃化冻存移植组(P<0.05);动情周期恢复需要的天数接近于新鲜移植组,明显短于未添加促卵泡刺激素的玻璃化冻存移植组(P<0.05).移植后4周,含促卵泡刺激素的玻璃化冻存移植组组织学观察见卵泡发育,未添加促卵泡刺激素的玻璃化冻存移植组仅偶见原始卵泡.含促卵泡刺激素的玻璃化冻存移植组与新鲜移植组相比血清雌二醇水平差异无显著性意义(P>0.05),显著高于未添加促卵泡刺激素的玻璃化冻存移植组(P< 0.05).结果提示,在玻璃化液中加入促卵泡刺激素可提高冻存绵羊卵巢组织移植后卵泡存活率.
揹景:卵巢皮質片移植是無血管吻閤移植,因此,提高卵巢組織對凍存-解凍和移植後缺血的耐受力是提高凍存後移植物卵泡存活和延長功能壽命的關鍵環節.目的:觀察促卵泡刺激素在玻璃化凍存過程中對綿羊卵巢組織形態和功能的保存效果,為成人卵巢組織的凍存提供技術方法.方法:BALB/c品繫雌性裸鼠隨機分為3組.均行羊卵巢皮質片裸鼠異位移植:①新鮮移植對照組,取材後即移植.②玻璃化凍存移植組,採用玻璃化凍存解凍後移植,所用液體均未添加促卵泡刺激素.③添加促卵泡刺激素的玻璃化凍存移植組,採用冷凍液、解凍液和培養液均添加促卵泡刺激素的玻璃化凍存後移植.移植後檢測受體鼠動情週期恢複率、恢複時間、卵泡數和髮育狀況,于移植後4週取移植卵巢進行組織學觀察、併行血清雌二醇水平分析.結果與結論:含促卵泡刺激素的玻璃化凍存移植組與新鮮移植組相比動情週期恢複率、每高倍視野卵泡計數差異均無顯著性意義(P>0.05),卵泡計數高于未添加促卵泡刺激素的玻璃化凍存移植組(P<0.05);動情週期恢複需要的天數接近于新鮮移植組,明顯短于未添加促卵泡刺激素的玻璃化凍存移植組(P<0.05).移植後4週,含促卵泡刺激素的玻璃化凍存移植組組織學觀察見卵泡髮育,未添加促卵泡刺激素的玻璃化凍存移植組僅偶見原始卵泡.含促卵泡刺激素的玻璃化凍存移植組與新鮮移植組相比血清雌二醇水平差異無顯著性意義(P>0.05),顯著高于未添加促卵泡刺激素的玻璃化凍存移植組(P< 0.05).結果提示,在玻璃化液中加入促卵泡刺激素可提高凍存綿羊卵巢組織移植後卵泡存活率.
배경:란소피질편이식시무혈관문합이식,인차,제고란소조직대동존-해동화이식후결혈적내수력시제고동존후이식물란포존활화연장공능수명적관건배절.목적:관찰촉란포자격소재파리화동존과정중대면양란소조직형태화공능적보존효과,위성인란소조직적동존제공기술방법.방법:BALB/c품계자성라서수궤분위3조.균행양란소피질편라서이위이식:①신선이식대조조,취재후즉이식.②파리화동존이식조,채용파리화동존해동후이식,소용액체균미첨가촉란포자격소.③첨가촉란포자격소적파리화동존이식조,채용냉동액、해동액화배양액균첨가촉란포자격소적파리화동존후이식.이식후검측수체서동정주기회복솔、회복시간、란포수화발육상황,우이식후4주취이식란소진행조직학관찰、병행혈청자이순수평분석.결과여결론:함촉란포자격소적파리화동존이식조여신선이식조상비동정주기회복솔、매고배시야란포계수차이균무현저성의의(P>0.05),란포계수고우미첨가촉란포자격소적파리화동존이식조(P<0.05);동정주기회복수요적천수접근우신선이식조,명현단우미첨가촉란포자격소적파리화동존이식조(P<0.05).이식후4주,함촉란포자격소적파리화동존이식조조직학관찰견란포발육,미첨가촉란포자격소적파리화동존이식조부우견원시란포.함촉란포자격소적파리화동존이식조여신선이식조상비혈청자이순수평차이무현저성의의(P>0.05),현저고우미첨가촉란포자격소적파리화동존이식조(P< 0.05).결과제시,재파리화액중가입촉란포자격소가제고동존면양란소조직이식후란포존활솔.
BACKGROUND: Transplantation of fragments of ovarian cortex is performed without vascular reanastomosis, therefore, to increase the tolerance of ovarian tissue to the freezing-thawing and ischemic injuries is critical for follicular survival and functional longevity of the graft.OBJECTIVE: To investigate the effect of follicle stimulating hormone (FSH) on the morphological and function of sheep ovary tissue in the process of cryopreservation, so that to provide new freezing method for human ovary tissues. METHODS: Healthy BALB/c strain female nude mice were equally and randomly divided into 3 groups and subjected to heterotopic transplantation of fragments of sheep ovarian cortex. (1) Control group: transplantation following sampling; (2) experimental group: transplantation following freezing-thawing, and the solution was free of FSH; (3) FSH group: the freezing and thawing and culture fluid contained FSH. The estrous cycle recovering rate, estrous cycle recovering time, the number of follicle were observed following transplantation. The histological changes, and the level of E2 in blood serum were observed at 4 weeks after transplantation.RESULTS AND CONCLUSION: There were no significant differences in estrous cycle recovering rate and number of follicle/PHF between FSH and control groups (P> 0.05), but the number of follicle was greater than the experimental group (P< 0.05). Moreover, the time of estrous cycle recovering in FSH group was similar to control group, but shorter than experimental group (P < 0.05). There were more developing follicular in FSH group, but few in experimental group at 4 weeks. No significant difference was detected in E2 level in blood serum between FSH and control group (P > 0.05), but significantly greater than the experimental group (P< 0.05). Results show that FSH addition in vitrification fluid can improve ovarian follicle survival following cryopreserved sheep ovary tissue transplantation.
