猕猴精子冷冻保存方法的改进及活率检测

精液的冷冻保存对家畜繁殖、人类辅助生殖以及濒危物种保护有着重要意义。然而目前精子冷冻的研究很大程度上是经验性的，并且要使用含卵黄、脱脂乳等复杂成分的稀释液。这些复杂成分不仅是潜在的污染源，也使精子冷冻中的质量控制及分析特定物质的功能变得困难。即便如此也仅有约50％的精子能够存活下来，而且存活精子的受精能力也有所下降。称猴是生物医学研究中使用广泛的灵长类动物，开展赫猴精子的冷冻保存有利于该物种的繁殖并促进基础胚胎学的研究，成功的称猴精子冷冻方法还可以为其它珍稀濒危灵长类动物所借鉴。但是目前成功的称猴精子冷冻的报道仍然很少，且精子质量检测方法并不完善。因此本文致力于建立简单有效的称猴精子冷冻方法和活率检测方法。主要结果如下：1）建立了一种用单一紫外激光同时激发Hoechst33342和碘化丙锭结合流式细胞术检测称猴精子活率的有效方法，并将此方法用于称猴精子冷冻研究。2）发现甘油的一步加入或去除与分步加入或去除对称猴精子冷冻效果没有明显影响，在此基础上发现各种糖类稀释液之间的作用差异很小，但不含糖的化学成分确定的TT稀释液对精子冷冻保护作用显著高于糖类稀释液。这可能是因为TT的渗透压（138mOsm/kg）较好地适合于猫猴精子的冻存，高渗毒害作用可能是导致称猴精子用TEST冷冻存活率低的重要原因。3）以TT为基础稀释液，探讨了精子冷冻中一些关键因素，以期进一步改进冷冻方法。结果表明精液一步稀释于含5％甘油的一倍浓度TT，平衡0.5h可得到最佳效果，总体上复苏精子的运动度可达到55％以上，质膜完整性能达到6D％左右。这种方法与传统的以含有卵黄的TTE为稀释液的称猴精子冷冻方法效果相当，复苏精子还能够成功地进行体外受精。另外，用液化精液1：2直接稀释于防冻液还能进一步提高冷冻效果。本研究建立的用化学成分确定稀释液冷冻称猴精子的简单方法，有利于提高称猴精子的冻存效率，并有助于分析特定成分在精子冷冻中的作用。而Hoechst33342和碘化丙锭双染方法，是一种简单有效的精子活率检测方法，并在多参数精子功能的流式检测中有很高应用价值。

灵长类动物精子超低温冷冻保存的研究

精子的超低温冷冻保存为珍稀、濒危动物种质资源的保存、人类不育症的治疗、家畜繁殖以及辅助生殖技术（如人工授精、体外受精和胚胎移植）的进一步发展奠定了基础。灵长类动物精子的冷冻保存距今已有30多年的历史，到目前为止，全世界两百余种灵长类动物中仅有约15个物种的精子被冷冻保存的报道，而用冷冻精液人工授精产下后代的报道仅见于大猩猩、黑猩猩、食蟹猴、械猴和称猴等5种灵长类动物。冻精人工授精率如此之低主要是因为人们对灵长类动物精子的低温生物学知识、精子的冷冻损伤机制以及某些物质的冷冻保护作用机理缺乏了解，导致了冷冻复苏精子的存活率降低，受精力急剧下降。为了探讨灵长类动物精子冷冻损伤的机理，提高精子的冷冻保存效率，本论文以食蟹猴和称猴为动物模型，以冷冻复苏精子的运动度、质膜完整率和顶体完整率为检测指标，对．影响灵长类动物精子冷冻保存效果的因素作了积极的探讨和研究：1）研究了脯氨酸、谷氨酞胺和甘氨酸对食蟹猴精子冷冻保存的影响，发现一定浓度的氨基酸有利于食蟹猴精子的冷冻保存，但高浓度的氨基酸却会对冷冻复苏精子产生负面影响；2）首次建立了灵长类动物精子成分确定防冻液的冷冻保存方法，为准确分析研究精子冷冻损伤机制和某些物质的冷冻保护机理莫定了基础；3）对比研究了不同类型冷冻保存稀释液及不同渗透性防冻剂在食蟹猴精子冷冻保存中的作用以及对冷冻复苏精子功能的影响，筛选、优化出了凡种适合于食蟹猴精子冷冻保存的稀释液和渗透性防冻剂；4）比较研究了几种不同类型防冻液对食蟹猴和称猴精子冷冻保存的效果，发现适合食蟹猴精子冻存的防冻液也同样适合于称猴精子。本研究的结果既有利于改进现有的灵长类动物精子冷冻保存方法，又有利于对精子的冷冻损伤机制和保护性物质的作用机理作进一步的研究，为低温生物学和生物多样性的保护作贡献。

猕猴精子的冷冻保存以及影响冷冻复苏精子功能的因素

自从1949年Polge等研究者发现甘油的冷冻保护作用，开创了低温生物学的里程碑以来，精子冷冻保存已经逐渐成为治疗人类不育、家畜繁殖和生物多样性保护的重要手段。然而目前人类对多数物种的基本生殖生物学及其种质冷冻保存的低温生物学知识仍很缺乏。哺乳动物精子冷冻的研究很大程度上是经验性的，即使运用最现代的低温冷冻程序和仪器设备，也仅有约50％的精子能够存活下来。灵长类动物的精子对冷冻非常敏感，迄今为止应用称猴冷冻精子人工受精仅产生过一个后代。为了提高冷冻保存精子的功能和受精能力，本论文以称猴为动物模型，以冷冻复苏精一的运动度、精子质膜和顶体的完整率以及体外受精作为精子功能的检钡l指标，探讨影响动物精子冷冻保存的因素。通过研究1）建立了适合称猴精子冷冻保存的适宜方法以及冷冻复苏精子功能的检测方法，并首次成功地运用冷冻称猴精子体外受精；2）检测了不同甘油浓度和二甲亚飒浓度对冷冻复苏精子运动能力、精子质膜、精子顶体结构和受精能力的影响，确定了称猴精子冷冻保存的适宜甘油浓度；3）对比研究了不同类型渗透性防冻剂在精子冷冻保存中的作用以及对冷冻复苏精子功能的影响，发现对于称猴精子，除了甘油外，乙二醇也是一种优秀的渗透性防冻剂，而丙二醇和二甲亚矾对精子产生了较大的毒害作用，并不适合称猴精子的冷冻保存；4）研究了单糖、二糖和二糖在精子冷冻复苏过程中的保护作用，发现不同类型糖类的冷冻保护作用存在显著差异，单糖和二糖对精子的冷冻保护作用优于二糖，二糖在冷冻复苏过程中对于精子的顶体产生了破坏作用，不同类型的糖类配合使用可以提高对精子的冷冻保护效率。本研究的结果有利于优化灵长类动物精子冷冻保存的方法，包括调整防冻液的成分和冷冻降温程序，从而有助于提高精子冷冻保存的存活率。此外，还有利于深入研究哺乳动物精子冷冻损伤的机制和探讨防冻剂的冷冻保护机理.

Effect of storage time and cryoprotectant concentrations on the fertilization rate and hatching rate of cryopreserved sperm in red seabream (Pagrus major Temminck & Schlegel, 1843)

This study examined the effects of storage time and cryoprotectant concentrations on the post-thaw sperm of red seabream, Pagrus major. Sperm treated with 12%, 15%, 18% and 21% DMSO were cryopreserved for 10, 30, 60 and 360 days, and fertilization and hatching rates were analysed. For all groups, there were no differences in the fertilization rates and hatching rates between sperm cryopreserved for < 60 days and fresh sperm (98.8 +/- 0.8%, 96.4 +/- 1.3%). However, for sperm cryopreserved for 360 days, both fertilization rates (88.6 +/- 3.0% to 7.0 +/- 1.9%) and hatching rates (79.4 +/- 7.2% to 3.3 +/- 0.8%) decreased drastically. Furthermore, the cryoprotectant concentrations affected sperm quality significantly (P < 0.05). When cryopreserved for 360 days, sperm treated with 15% DMSO obtained the best results compared with other concentrations. We suggest that 15% DMSO may be an effective cryoprotectant for long-term sperm cryopreservation of red seabream.

Extra- and intra-cellular ice formation of red seabream (Pagrus major) embryos at different cooling rates

The ice crystal formation is assumed as the most lethal factor for the failure of fish embryo cryopreservation and intracellular ice formation (IIF) plays a central role in cell injury during cooling. The objectives were to observe the morphological changes of red seabream (Pagrus major) embryo during the cooling-thawing process, and to examine the effect of cryoprotectant and cooling rate on the temperatures of oil globule ice formation (T-OIF), extra-cellular ice formation (T-EIF) and intracellular ice formation (T-IIF) using cryomicroscope. After thawing, the morphological changes of embryos were observed and recorded by the video attachment and monitor under the microscope. During the cooling process, three representative phenomena were observed: oil globule gradually turned bright firstly, then the whole field of view flashed and the embryo blackened. Cooling rate affect the temperature of both extra- and intra-cellular ice formations. T-EIF and T-IIF at high cooling rate were much lower than that at low cooling rate. And the value of T-EIF - T-IIF increased from 0.45 to 11.11 degrees C with the increase of cooling rate from 3 to 130 degrees C/min. Taken together, our results suggested that high cooling rate with proper cryoprotectant would be a good option for red seabream embryo cryopreservation. (C) 2009 Elsevier Inc. All rights reserved.

Toxicity and protective efficiency of cryoprotectants to flounder (Paralichthys olivaceus) embryos

With the purpose of finding an ideal cryoprotectant or combination of cryoprotectants in a suitable concentration for flounder (Paralichthys olivaceus) embryo cryopreservation, we tested the toxicities, at culture temperature (16 degrees C), of five most commonly used cryoprotectants-dimethyl sulfoxide (Me2SO), glycerol, methanol (MeOH), 1,2-propylene glycol (PG) and ethylene glycol (EG). In addition, cryoprotective efficiency to flounder embryos of individual and combined cryoprotectants were tested at -15 degrees C for 60 min. Five different concentrations of each of the five cryoprotectants and 20 different combinations of these cryoprotectants were tested for their protective efficiency. The results showed that the toxicity to flounder embryos of the five cryoprotectants are in the following sequence: PG < MeOH < Me2SO < glycerol < EG (P < 0.05); whereas the protective efficiency of each cryoprotectant, at -15 degrees C for a period of 60 min, are in the following sequence: PG > Me2SO approximate to MeOH approximate to glycerol > EG (greater symbols mean P < 0.05, and approximate symbols mean P > 0.05). Methanol combined with any one of the other cryoprotectants gave the best protection, while ethylene glycol combined with any one of the other cryoprotectants gave the poorest protection at -15 degrees C. Toxicity effect was concentration dependent with the lowest concentration being the least toxic for all five cryoprotectants at 16 degrees C. For PG, MeOH and glycerol, 20% solutions gave the best protection at -15 degrees C; whereas a 15% solution of Me2SO, and a 10% solution of EG, gave the best protection at -15 degrees C. (c) 2004 Elsevier Inc. All rights reserved.

真鲷（Pagrus major）胚胎超低温损伤机理研究

鱼类胚胎由于其自身结构特征：体积大、含水量高、多室结构等，迄今超低温保存尚未成功。超低温保存过程中所造成的冷冻损伤是制约鱼类胚胎超低温保存成功与否的关键，具体表现为渗透压影响、抗冻剂毒性、冰晶损伤等。系统研究并阐明鱼类胚胎冷冻损伤机理，是成功建立鱼类胚胎超低温保存技术的基础。本论文主要针对胚胎对渗透压的耐受性、抗冻剂对胚胎的渗透性、降温速率对胚胎内外冰晶形成温度的影响等冷冻损伤机理进行了系统研究，主要研究结果如下： 1.通过检测胚胎在不同浓度人工海水（0%、25%、50%、75%、1×、2×、3×、4×，渗透压范围0~3740 mOsm/kg）中的孵化率，确定了真鲷不同发育时期胚胎对渗透压的耐受范围，以及心跳期胚胎浸泡不同时间对渗透压的耐受范围。结果显示：①真鲷2-4细胞期、原肠期、10-14体节期胚胎、心跳期和出膜前期胚胎孵化率>50%时渗透压的范围依次为：919~1391 mOsm/kg、919~1391 mOsm/kg、462 ~1391 mOsm/kg、232~1878 mOsm/kg和692~1391 mOsm/kg，表明心跳期胚胎对渗透压变化的耐受范围最广；②在不同浓度人工海水中分别浸泡10 min、30 min、1 h、5 h和10 h后，真鲷胚胎孵化率无显著变化的渗透压范围分别为0~2804 mOsm/kg、0~1878 mOsm/kg、232~1391 mOsm/kg、232~1391 mOsm/kg和919~1391 mOsm/kg；结果表明心跳期胚胎对渗透压的耐受范围随浸泡时间的延长而减小。 2.采用毛细管电泳技术检测胚胎内部DMSO的浓度，并且分析了胚胎孵化率和胚胎内部DMSO的浓度随浸泡时间变化与外部抗冻剂的关系。结果表明胚胎孵化率随胚胎外部抗冻剂溶液浓度和浸泡时间的增加而降低；胚胎内部DMSO浓度随胚胎外部抗冻剂溶液浓度和浸泡时间的增加而增加。对胚胎孵化率（y1）随抗冻剂溶液浓度（x）的变化进行一元三次多项式回归，当浸泡时间分别为10 min、30 min和60 min时，回归方程依次为：y1 = -2832.7x3 + 575.01x2 - 37.011x + 99.641（R2 = 0.9722）；y1 = 30288x3 - 16322x2 + 2077.3x + 27.603（R2 = 0.9876）；y1 = 16052x3 - 5985.2x2 - 32.696x + 119.6（R2 = 0.9124）。对胚胎内部DMSO浓度（y2）随抗冻剂溶液浓度（x）的变化进行回归，当浸泡时间分别为10 min、30 min和60 min时，回归方程依次为：y2 = 0.2584e6.7294x（R2 = 0.9876）；y2 = 0.2521e10.964x（R2 = 0.9644）；y2 = 0.4054e10.95x（R2 = 0.8954）。 3. 利用低温显微镜观察了不同降温速率（20、40、60、80、100、120℃/min）对胚胎内外冰晶形成温度的影响。胚胎外部冰晶形成温度（TEIF）随降温速率的增加显著下降，在降温速率大于80℃/min之后，TEIF随降温速率增加而降低的幅度减小；胚胎内部冰晶形成温度（TIIF）在降温速率小于80℃/min 时随降温速率的升高而降低，在降温速率大于80℃/min 时随降温速率的升高而升高；胚胎内外冰晶形成温度差值（TEIF - TIIF）在降温速率小于80℃/min时随降温速率的升高而增大，在降温速率大于80℃/min时随降温速率的升高而减小。 4. 在低温显微镜下观察了真鲷胚胎低温保存中有复活胚胎记录的保存方法在冷冻解冻过程中的冰晶形成过程，结果表明：①在冷冻过程中，玻璃化法冷冻的胚胎的内部冰晶形成温度（-53.70，-64.33℃）显著低于程序降温法（-17.51，-21.40℃）；而且在玻璃化法冷冻的胚胎内部冰晶形成温度高于外部冰晶后形成（-70.30℃），程序降温法中则相反，胚胎内部冰晶形成温度显著低于外部冰晶形成温度（-4.93，-5.00℃）；玻璃化法中，40%PG冷冻的胚胎外部溶液出现玻璃化现象，其他组均未出现；②在解冻过程中，各组均出现重结晶现象；解冻后，玻璃化法的胚胎完整率（62.82%）远高于程序降温法（9.21%）。

大西洋庸鲽Hippoglossus hippoglossus和大西洋鲑Salmo salar配子质量研究

种质问题是养殖健康发展的基础。在鱼类养殖中，卵子和精子的质量直接关系到受精、胚胎发育，仔稚鱼发育以及幼鱼生长等一系列过程。本论文针对大西洋庸鲽和大西洋鲑的配子质量进行研究。研究内容涉及大西洋庸鲽精子冷冻保存方法；促性腺激素释放激素类似物（GnRHa）使用对其精子冷冻保存效果、以及脂肪酸组成的影响；野生和驯养大西洋鲑卵子在脂肪酸、类胡萝卜素、矿物盐方面的差异比较。 精子冷冻保存通过提高对精子的利用效率，进而对于种质改良，推进鱼类养殖科研和生产具有重要意义。本实验建立了大西洋庸鲽精子大容量冷冻保存方法。八种抗冻剂冷冻保存实验结果表明：10% 及15% DMSO配以 HBSS 或KS 的抗冻剂组合冷冻保存效果最佳，4 mL体积冷冻保存可获得与1.6 mL同样的保存效果。 在繁殖季节后期注射GnRHa激素缓释剂，可获得质量稳定的大西洋庸鲽精液，将激素注射方法与精子冷冻保存方法相结合对于提高雄鱼利用率，扩大生产规模具有重要实用价值。本项研究分三个时间采集注射GnRHa激素后的雄鱼精子以及同期未注射激素的雄鱼精子，对所有精子样品使用同样的方法进行冷冻保存，检测冷冻保存后解冻精子的受精率与活力。结果表明，激素注射与否对于冷冻保存后精子的受精率和活力无显著影响，两类冷冻精液均达到鲜精水平。实验结果还表明，注射激素14天后的精子的密度显著的降低。说明GnRHa激素的使用可以显著降低精子密度，但不会影响精子的冷冻保存效果。 本相研究同时对注射GnRHa 缓释激素和未注射GnRHa 缓释激素的大西洋庸鲽精液脂肪酸成分进行分析，以检测该激素使用对精子生化组分的影响。结果表明激素的使用对在DHA (22:6n-3,二十二碳六烯酸)、EPA(20:5n-3,二十碳五烯酸)、AA(20:4n-6，花生四烯酸)等重要脂肪酸，不饱和脂肪酸、饱和脂肪酸以及n-3、n-6等重要种类的脂肪酸总量及其比例没有显著影响。精液脂肪酸中DHA含量最高，约占25%；PUFA约为44%。 作为世界性的重要养殖品种，野生和驯养大西洋鲑在形态、生化组成以及遗传 等方面表现出的差异被广泛关注。本论文，对野生和驯养大西洋鲑受精卵关键生化成分进行分析，通过与野生受精卵比较阐明驯养受精卵的质量状况，为亲鱼营养需求提供指导依据。本实验中野生配子和驯养配子的受精率没有显著差异，但重要脂肪酸组成、类胡萝卜素以及矿物盐含量都存在多方面显著差异。两类受精卵脂肪酸中含量最高的依次为18:1n-9（油酸）、DHA（二十二碳六烯酸）、16:0（棕榈酸）、EPA（二十碳五烯酸）。野生受精卵的单不饱和脂肪酸总量显著高于驯养受精卵，而多不饱和脂肪酸（PUFA）比例显著低于驯养的受精卵。在主要必需不饱和脂肪酸（EFA）中，DHA和EPA在野生受精卵中的比例高于驯养受精卵，AA（花生四烯酸）低于驯养受精卵。野生受精卵虾青素（Ax）的含量低于驯养受精卵而鸡油菌素（Cx）含量高于驯养受精卵。野生受精卵中多种矿物盐的含量（铝、铜、铁、硒和锌）含量显著高于驯养的受精卵。差别最大的为铜。诸多方面的差异表明，野生亲鱼与驯养亲鱼产出的卵子确实存在显著差异，因此关注亲鱼的营养极为重要。

Flow cytometry and ultrastructure of cryopreserved red seabream (Pagrus major) sperm

The objectives were to assess motility, fertilizing capacity, structural integrity, and mitochondrial function in fresh versus frozen-thawed (15% DMSO was used as a cryoprotectant) sperm from red seabrearn (Pagrus major). Mean (+/- S.D.) rates of motility, fertilization and hatching of frozen-thawed sperm were 81.0 +/- 5.4, 92.8 +/- 1.9, and 91.8 +/- 5.2%, respectively; for fresh sperm, they were 87.5 +/- 7.7, 95.8 +/- 2.4, and 93.8 +/- 4.2%. Although motility was lower in frozen-thawed versus fresh sperm (P < 0.05), there was no effect (P > 0.05) of cryopreservation on fertilization or hatching. Based on scanning and transmission electron microscopy, 77.8 +/- 5.6% of fresh sperm had normal morphology, whereas for frozen-thawed sperm, 63.0 +/- 7.2% had normal morphology, 20.6 +/- 3.1% were slightly damaged (e.g. swelling or rupture of head, mid-piece and tail region as well as mitochondria), and 16.4 +/- 4.2% were severely damaged. Sperm were stained with propidium iodide and Rhodamine 123 to assess plasma membrane integrity and mitochondrial function, respectively, and examined with flow cytometry. For fresh sperm, 83.9% had an intact membrane and functional mitochondria, whereas for frozen-thawed sperm, 74.8% had an intact membrane and functional mitochondria, 12.7% had a damaged membrane, 9.9% had nonfunctional mitochondria, and 2.6% had both a damaged membrane and nonfunctional mitochondria. In conclusion, ultrastructure and flow cytometry were valuable for assessment of frozen-thawed sperm quality; cryopreservation damaged the sperm but fertilizing ability was not significantly decreased. (c) 2007 Elsevier Inc. All rights reserved.

Use of computer-assisted sperm analysis (CASA) to evaluate the quality of cryopreserved sperm in red seabream (Pagrus major)

In the present study, the quality of post-thaw sperm of red seabream Pagrus major frozen with 6-24% DMSO was investigated. The motility, average path velocity and fertilizing capacity of fresh and their corresponding post-thaw sperm were examined for evaluation of the post-thaw sperm motion characteristics and its association with fertilizing capacity. An analysis of sperm motility before and after cryopreservation has been performed using computer-assisted sperm analysis (CASA). For post-thaw sperm frozen with 12-21% DMSO, the percentages of motile sperm were not significantly (P > 0.05) changed 10 s after activation. Moreover, the main motility pattern and swimming velocity of the motile post-thaw sperm were not significantly (P > 0.05) changed and the progressive linear motion was still the dominant pattern. However, the total motility of post-thaw sperm (72.3 +/- 6.3%) 30 s after activation was (P < 0.05) lower than the corresponding fresh sperm (82.7 +/- 7.2%). Additionally, the fertilizing capacity of post-thaw sperm was investigated with a standardized sperm to egg ratio 500:1. There is a linear regression relationship between the percentage of motile post-thaw sperm and fertilizing capability. These data demonstrate that 12-21% DMSO can provide good protection to the sperm during the freezing-thawing process. (c) 2006 Elsevier B.V. All rights reserved.

Fertility preservation: Successful transplantation of cryopreserved ovarian tissue in a young patient previously treated for Hodgkin's disease

Cryopreservation of ovarian tissue is now offered as an experimental procedure to preserve the fertility of young patients with a high risk for premature ovarian failure resulting from cancer therapy. This is the only available option to preserve the fertility of prepubertal patients treated with gonadotoxic chemotherapy. At present, thousands of patients all over the world have undergone this procedure with the hope of later restoring their fertility. Although the efficiency of the transplantation of cryopreserved ovarian tissue to restore ovarian function has been established, reports of pregnancy are still very scarce. Here, we describe the second published full-term spontaneous pregnancy after an orthotopic and heterotopic transplantation of cryopreserved ovarian tissue in a 31-year-old woman previously treated by conditioning therapy for bone marrow transplantation for Hodgkin's disease. This birth gives compelling evidence for the graft origin of the gamete and confirms the efficacy of ovarian tissue transplantation in restoring human natural fertility after oncological treatment. This case report stresses the importance of proposing the ovarian tissue cryopreservation procedure to all young patients who require potentially sterilizing treatment, with all alternative options to preserve fertility being duly taken into consideration.

Antigen-specific responses assessment for the evaluation of Bordetella pertussis T cell immunity in humans.

Measurement of antigen-specific T cell responses is an adjunctive parameter to evaluate protection induced by a previous Bordetella pertussis infection or vaccination. The assessment of T cell responses is technically complex and usually performed on fresh peripheral blood mononuclear cells (PBMC). The objective of this study was to identify simplified methods to assess pertussis specific T cell responses and verify if these assays could be performed using frozen/thawed (frozen) PBMC. Three read-outs to measure proliferation were compared: the fluorescent dye 5,6-carboxylfluorescein diacetate succinimidyl ester (CFSE) dilution test, the number of blast cells defined by physical parameters, and the incorporation of (3)H-thymidine. The results of pertussis-specific assays performed on fresh PBMC were compared to the results on frozen PBMC from the same donor. High concordance was obtained when the results of CFSE and blast read-outs were compared, an encouraging result since blast analysis allows the identification of proliferating cells and does not require any use of radioactive tracer as well as any staining. The results obtained using fresh and frozen PBMC from the same donor in the different T cell assays, including IFNγ and TNFα cytokine production, did not show significant differences, suggesting that a careful cryopreservation process of PBMC would not significantly influence T cell response evaluation. Adopting blast analysis and frozen PBMC, the possibility to test T cell responses is simplified and might be applied in population studies, providing for new instruments to better define correlates of protection still elusive in pertussis.

Electron tomography of cryofixed, isometrically contracting insect flight muscle reveals novel actin-myosin interactions.

BACKGROUND: Isometric muscle contraction, where force is generated without muscle shortening, is a molecular traffic jam in which the number of actin-attached motors is maximized and all states of motor action are trapped with consequently high heterogeneity. This heterogeneity is a major limitation to deciphering myosin conformational changes in situ. METHODOLOGY: We used multivariate data analysis to group repeat segments in electron tomograms of isometrically contracting insect flight muscle, mechanically monitored, rapidly frozen, freeze substituted, and thin sectioned. Improved resolution reveals the helical arrangement of F-actin subunits in the thin filament enabling an atomic model to be built into the thin filament density independent of the myosin. Actin-myosin attachments can now be assigned as weak or strong by their motor domain orientation relative to actin. Myosin attachments were quantified everywhere along the thin filament including troponin. Strong binding myosin attachments are found on only four F-actin subunits, the "target zone", situated exactly midway between successive troponin complexes. They show an axial lever arm range of 77°/12.9 nm. The lever arm azimuthal range of strong binding attachments has a highly skewed, 127° range compared with X-ray crystallographic structures. Two types of weak actin attachments are described. One type, found exclusively in the target zone, appears to represent pre-working-stroke intermediates. The other, which contacts tropomyosin rather than actin, is positioned M-ward of the target zone, i.e. the position toward which thin filaments slide during shortening. CONCLUSION: We present a model for the weak to strong transition in the myosin ATPase cycle that incorporates azimuthal movements of the motor domain on actin. Stress/strain in the S2 domain may explain azimuthal lever arm changes in the strong binding attachments. The results support previous conclusions that the weak attachments preceding force generation are very different from strong binding attachments.

Ovarian function and spontaneous pregnancy after combined heterotopic and orthotopic cryopreserved ovarian tissue transplantation in a patient previously treated with bone marrow transplantation: case report

Cryopreservation of ovarian tissue has been proposed for storing gametes of young patients at high risk of premature ovarian failure. Autotransplantation has recently provided some promising results and is still the unique option to restore ovarian function from cryopreserved ovarian tissue in humans. In this article, we analyse data from the combined orthotopic and heterotopic transplantation of cryopreserved ovarian tissue that restored the ovarian function and fertility. Orthotopic transplantation of cryopreserved ovarian tissue at ovarian and peritoneal sites, together with a heterotopic transplantation at the abdominal subcutaneous site, was performed to restore the ovarian function of a 29-year-old woman previously treated with bone marrow transplantation (BMT) for Hodgkin's disease. Ovarian reserve markers progressively suppress within values 5 months after the transplantation (basal FSH 5 mUI/ml and inhibin B 119 ng/ml). Follicular development was observed at all transplantation sites but was predominant at the ovarian site. Six natural cycles were fully documented and analysed. The patient became spontaneously pregnant following the sixth cycle, but unfortunately she later miscarried. Combined orthotopic and heterotopic transplantations succeeded in the restoration of normal spontaneous cycles. Furthermore, this spontaneous pregnancy confirmed the efficiency of this procedure for restoring human fertility.

The effects of short and long incubations on DNA fragmentation of testicular

DNA fragmentation in testicular sperm from men with obstructive azoospermia is increased by 4 hr and 24 hr incubations, and after cryopreservation. The effect is intensified by post-thaw incubations. Testicular sperm to be used clinically in ICSI should be injected without delay.