Ganguli Nirmalya, Wadhwa Neerja, Usmani Abul, Kunj Neetu, Ganguli Nilanjana, Sarkar Rajesh Kumar, Ghorai Soma M, Majumdar Subeer S
Embryo Biotechnology Laboratory, National Institute of Immunology, Aruna Asaf Ali Marg, New Delhi, 110067, India.
Department of Zoology, University of Delhi, Delhi, 110 007, India.
Stem Cell Res Ther. 2016 Sep 22;7(1):142. doi: 10.1186/s13287-016-0405-1.
Spermatogonial stem cell (SSC) transplantation (SSCT) has become important for conservation of endangered species, transgenesis and for rejuvenating testes which have lost germ cells (Gc) due to gonadotoxic chemotherapy or radiotherapy during the prepubertal phase of life. Creating a germ cell-depleted animal model for transplantation of normal or gene-transfected SSC is a prerequisite for such experimental studies. Traditionally used intraperitoneal injections of busulfan to achieve this are associated with painful hematopoietic toxicity and affects the wellbeing of the animals. Use of testicular busulfan has been reported recently to avoid this but with a very low success rate of SSCT. Therefore, it is necessary to establish a more efficient method to achieve higher SSCT without any suffering or mortality of the animals.
A solution of busulfan, ranging from 25 μg/20 μl to 100 μg/20 μl in 50 % DMSO was used for this study. Each testis received two diagonally opposite injections of 10 μl each. Only DMSO was used as control. Germ cell depletion was checked every 15 days. GFP-expressing SSC from transgenic donor mice C57BL/6-Tg (UBC-GFP) 30Scha/J were transplanted into busulfan-treated testis. Two months after SSCT, mice were analyzed for presence of colonies of donor-derived SSC and their ability to generate offspring.
A dose of 75 μg of busulfan resulted in reduction of testis size and depletion of the majority of Gc of testis in all mice within 15 days post injection without causing mortality or a cytotoxic effect in other organs. Two months after SSCT, colonies of donor-derived Gc-expressing GFP were observed in recipient testes. When cohabitated with females, donor-derived offspring were obtained. By our method, 71 % of transplanted males sired transgenic progeny as opposed to 5.5 % by previously described procedures. About 56 % of progeny born were transgenic by our method as opposed to 1.2 % by the previously reported methods.
We have established an efficient method of generating a germ cell-depleted animal model by using a lower dose of busulfan, injected through two diagonally opposite sites in the testis, which allows efficient colonization of transplanted SSC resulting in a remarkably higher proportion of donor-derived offspring generation.
精原干细胞(SSC)移植(SSCT)对于濒危物种的保护、转基因研究以及使因青春期前阶段性腺毒性化疗或放疗而失去生殖细胞(Gc)的睾丸恢复活力而言已变得至关重要。创建一个用于移植正常或基因转染的SSC的生殖细胞耗竭动物模型是此类实验研究的先决条件。传统上用于实现这一目的的腹腔注射白消安会带来痛苦的造血毒性,并影响动物的健康。最近有报道称使用睾丸内注射白消安可避免此问题,但SSCT的成功率非常低。因此,有必要建立一种更有效的方法,以在不造成动物任何痛苦或死亡的情况下实现更高的SSCT成功率。
本研究使用了浓度范围为25μg/20μl至100μg/20μl的白消安溶液,该溶液以50%二甲基亚砜(DMSO)配制。每个睾丸接受两次对角相对的注射,每次注射10μl。仅使用DMSO作为对照。每15天检查一次生殖细胞耗竭情况。将来自转基因供体小鼠C57BL/6-Tg(UBC-GFP)30Scha/J的表达绿色荧光蛋白(GFP)的SSC移植到经白消安处理过的睾丸中。SSCT两个月后,分析小鼠体内供体来源的SSC集落的存在情况及其产生后代的能力。
75μg白消安的剂量导致所有小鼠在注射后15天内睾丸体积减小且大部分睾丸生殖细胞耗竭,同时未导致死亡或对其他器官产生细胞毒性作用。SSCT两个月后,在受体睾丸中观察到了供体来源的表达GFP的生殖细胞集落。当与雌性小鼠同居时,可以获得供体来源的后代。通过我们的方法,71%的移植雄性小鼠产生了转基因后代,而之前描述的方法这一比例为5.5%。通过我们的方法出生的后代中约56%为转基因后代,而之前报道的方法这一比例为1.2%。
我们建立了一种有效的方法,通过在睾丸中两个对角相对的部位注射较低剂量的白消安来创建生殖细胞耗竭动物模型,这使得移植的SSC能够有效定植,从而产生供体来源后代的比例显著更高。
Zotero 插件
