Single-cell analysis comparing early-stage oocytes from fresh and slow-frozen/thawed human ovarian cortex reveals minimal impact of cryopreservation on the oocyte transcriptome.

IF 6 1区医学 Q1 OBSTETRICS & GYNECOLOGY

Human reproduction Pub Date : 2025-04-01 DOI:10.1093/humrep/deaf009

J H Machlin, D F Hannum, A S K Jones, T Schissel, K Potocsky, E E Marsh, S Hammoud, V Padmanabhan, J Z Li, A Shikanov

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Clinical cases reported in the past 10 years have demonstrated that transplanted slow-frozen/thawed and fresh ovarian cortex restored normal serum FSH levels and regular menstrual cycles by 5 months. However, the slow-frozen and thawed tissue resulted in lower rates of pregnancies and live births, albeit not statistically significant.Study design, size, duration: We utilized single-cell RNA-sequencing (scRNAseq) of 144 human oocytes isolated from cadaver ovaries obtained from three donors.Participants/materials, setting, methods: Human ovarian cortex from three healthy premenopausal donors 16, 18, and 27 years old was cut into squares measuring 10 × 10 × 1 mm3 and either slow-frozen and thawed or processed fresh. First, using a novel method for isolating live oocytes from primordial and primary follicles, the ovarian cortex squares were fragmented with a McIlwain tissue chopper and enzymatically digested. Next, oocytes were mechanically denuded under a dissection microscope and placed individually into wells containing lysis buffer for scRNAseq. Lysed single oocytes were subjected to library prep using the seqWell PlexWell rapid single-cell RNA protocol. Pooled libraries were subjected to 150-bp paired-end sequencing on the NovaSeq6000 Illumina platform. In total, we sequenced 144 oocytes-24 oocytes isolated fresh and 24 oocytes isolated after slow-freezing and thawing from each of the three donors. 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引用次数: 0

Abstract

Study question: Does the slow-freezing and thawing process have a negative impact on the transcriptome of oocytes isolated from early-stage human follicles compared to fresh controls?

Summary answer: The transcriptional profiles of fresh and frozen/thawed oocytes did not cluster separately, indicating undetectable differences between the two groups when compared to within-donor heterogeneity.

What is known already: Previous studies using histological analysis of follicle morphology, density, and stage distribution in slow-frozen/thawed human ovarian cortex compared to fresh controls showed no differences between the two groups. Clinical cases reported in the past 10 years have demonstrated that transplanted slow-frozen/thawed and fresh ovarian cortex restored normal serum FSH levels and regular menstrual cycles by 5 months. However, the slow-frozen and thawed tissue resulted in lower rates of pregnancies and live births, albeit not statistically significant.

Study design, size, duration: We utilized single-cell RNA-sequencing (scRNAseq) of 144 human oocytes isolated from cadaver ovaries obtained from three donors.

Participants/materials, setting, methods: Human ovarian cortex from three healthy premenopausal donors 16, 18, and 27 years old was cut into squares measuring 10 × 10 × 1 mm3 and either slow-frozen and thawed or processed fresh. First, using a novel method for isolating live oocytes from primordial and primary follicles, the ovarian cortex squares were fragmented with a McIlwain tissue chopper and enzymatically digested. Next, oocytes were mechanically denuded under a dissection microscope and placed individually into wells containing lysis buffer for scRNAseq. Lysed single oocytes were subjected to library prep using the seqWell PlexWell rapid single-cell RNA protocol. Pooled libraries were subjected to 150-bp paired-end sequencing on the NovaSeq6000 Illumina platform. In total, we sequenced 144 oocytes-24 oocytes isolated fresh and 24 oocytes isolated after slow-freezing and thawing from each of the three donors. Additionally, we performed histological analysis of fresh and frozen/thawed ovarian cortex tissue from all three donors using hematoxylin and eosin staining and analyzed morphology, follicle density, and follicle stage distribution differences between fresh and cryopreserved ovarian cortex.

Main results and the role of chance: The histological analysis revealed no differences in follicle stage distribution or follicle morphology between conditions, with the percentage of normal follicles in fresh and frozen/thawed tissue, respectively, as 86.7% and 91.0% for Donor 1, 91.7% and 92.5% for Donor 2, and 96.1% and 91.1% for Donor 3. The follicle density per mm3 in fresh and frozen/thawed tissue, respectively, was 279.4 and 235.8 for Donor 1, 662.2 and 553.5 for Donor 2, and 55.8 and 71.4 for Donor 3. The difference in follicle density was not statistically significant between fresh and frozen/thawed conditions for Donors 2 and 3, and significant (P = 0.017) for Donor 1. The stromal cell densities in fresh and frozen/thawed tissue, respectively, were 0.014 in both conditions for Donor 1, 0.014 and 0.016 for Donor 2, and 0.013 and 0.014 for Donor 3. There was no statistically significant difference in stromal cell density between conditions in Donor 1 and Donor 3, though it was statistically significant (P ≤ 0.001) for Donor 2. The transcriptional profiles of fresh and frozen/thawed oocytes did not cluster separately, suggesting insignificant differences between the two groups. However, at the group mean level, there was a small shift between the fresh and frozen/thawed oocytes and the shifts were parallel across the three donors. In this comparison, fresh oocytes were enriched for gene ontology terms related to chromosome segregation and mitosis, whereas frozen/thawed oocytes were enriched for terms related to wound response, cAMP signaling, and extracellular matrix organization.

Large scale data: Datasets available on Zenodo.org. DOI: https://zenodo.org/records/13224872.

Limitations, reasons for caution: In this study, we only sequenced the oocytes isolated from early-stage follicles due to technical challenges collecting and sequencing the somatic cells surrounding the oocytes. Investigating the transcriptomic changes after freezing and thawing in the somatic cells would need to be studied in the future. Additionally, we built RNAseq libraries immediately after thawing focusing on the immediate changes. Investigation of the effects that manifest at later timepoints, either in culture or upon implantation in an animal model, may reveal additional effects of the freeze/thaw process on the transcriptome.

Wider implications of the findings: The only clinically approved method of fertility preservation for prepubertal cancer patients and adult patients who cannot delay cancer treatment is ovarian tissue cryopreservation. Investigation of cryopreservation-induced changes in follicles at all stages is critical to further our understanding of the safety and efficacy of using these tissues for fertility preservation in the clinic. Our study is the first to analyze transcriptomic changes between individual fresh and slow-frozen/thawed human oocytes collected from early-stage follicles. To accomplish this, we developed a novel method for dissociating both fresh and frozen/thawed human ovarian cortex to obtain live denuded oocytes from early-stage follicles. Our findings provide insights into the use of cryopreserved tissue and follicles for fertility preservation efforts.

Study funding/competing interest(s): This work was funded by National Institutes of Health (NIH) R01HD099402, Career Training in Reproductive Biology (CTRB) Training Grant National Institutes of Health (NIH) T32 to Jordan Machlin, National Institutes of Health (NIH) F31-HD106626 and National Institutes of Health (NIH) T31H-D079342 to Andrea Jones, National Institutes of Health (NIH) T32-GM70449 to D. Ford Hannum, and The Chan Zuckerberg Initiative Grant CZF2019-002428. We have no conflicts of interest to declare.

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比较新鲜和缓慢冷冻/解冻人卵巢皮层的早期卵母细胞的单细胞分析显示，冷冻保存对卵母细胞转录组的影响最小。

研究问题：与新鲜对照相比，缓慢冷冻和解冻过程是否对从早期人类卵泡中分离的卵母细胞的转录组有负面影响？摘要回答：新鲜和冷冻/解冻卵母细胞的转录谱没有单独聚集，表明与供体内异质性相比，两组之间存在不可检测的差异。已知情况：先前的研究使用慢速冷冻/解冻人类卵巢皮层的卵泡形态、密度和分期分布的组织学分析，与新鲜对照相比，两组之间没有差异。过去10年的临床病例报告表明，移植的缓慢冷冻/解冻和新鲜卵巢皮质可使正常血清FSH水平和正常月经周期恢复5个月。然而，缓慢冷冻和解冻的组织导致较低的怀孕率和活产率，尽管在统计上没有显著性。研究设计、规模、持续时间：我们利用单细胞rna测序（scRNAseq）对从三个供体的尸体卵巢中分离的144个人卵母细胞进行测序。参与者/材料、环境、方法：来自3名健康的绝经前供体（分别为16、18和27岁）的人卵巢皮质被切成10 × 10 × 1 mm3大小的正方形，缓慢冷冻和解冻或新鲜加工。首先，采用一种从原始卵泡和初代卵泡中分离活卵母细胞的新方法，用McIlwain组织剪切器将卵巢皮质方形碎片化并酶解。接下来，在解剖显微镜下机械剥离卵母细胞，并将其单独放入含有裂解缓冲液的孔中。裂解的单个卵母细胞使用seqWell PlexWell快速单细胞RNA协议进行文库准备。汇集的文库在NovaSeq6000 Illumina平台上进行150 bp的配对端测序。我们总共测序了144个卵母细胞，其中24个是新鲜分离的卵母细胞，24个是缓慢冷冻和解冻后分离的卵母细胞。此外，我们使用苏木精和伊红染色对所有三位供者的新鲜和冷冻/解冻卵巢皮质组织进行组织学分析，并分析新鲜和冷冻保存卵巢皮质的形态学、卵泡密度和卵泡分期分布差异。主要结果及偶发因素的作用：组织学分析显示，不同条件下卵泡分期分布和卵泡形态无差异，供体1和冷冻/解冻组织中正常卵泡的百分比分别为86.7%和91.0%，供体2和冷冻/解冻组织中正常卵泡的百分比分别为91.7%和92.5%，供体3和91%和91.1%。在新鲜和冷冻/解冻组织中，供体1的卵泡密度分别为279.4和235.8，供体2为662.2和553.5，供体3为55.8和71.4。供体2和供体3的卵泡密度在新鲜和冷冻/解冻条件下差异无统计学意义，供体1的差异有统计学意义（P = 0.017）。供体1和供体2的基质细胞密度分别为0.014和0.016，供体3的基质细胞密度分别为0.013和0.014。供体1和供体3间质细胞密度差异无统计学意义，供体2间质细胞密度差异有统计学意义（P≤0.001）。新鲜卵母细胞和冷冻/解冻卵母细胞的转录谱没有单独聚集，表明两组之间差异不显著。然而，在组平均水平上，新鲜卵母细胞和冷冻/解冻卵母细胞之间的变化很小，并且在三个供体之间的变化是平行的。在这个比较中，新鲜卵母细胞富集了与染色体分离和有丝分裂相关的基因本体术语，而冷冻/解冻卵母细胞富集了与伤口反应、cAMP信号和细胞外基质组织相关的术语。大规模数据：Zenodo.org上提供的数据集。DOI: https://zenodo.org/records/13224872.Limitations，谨慎的原因：在这项研究中，由于收集和测序卵母细胞周围的体细胞的技术挑战，我们只对从早期卵泡中分离的卵母细胞进行了测序。研究体细胞冷冻和解冻后转录组学的变化需要在未来进行研究。此外，我们在解冻后立即构建RNAseq库，重点关注即时变化。研究在培养或植入动物模型的后期时间点所表现出的影响，可能会揭示冻结/解冻过程对转录组的其他影响。研究结果的广泛意义：唯一临床批准的保存青春期前癌症患者和不能延迟癌症治疗的成年患者生育能力的方法是卵巢组织冷冻保存。研究冷冻保存在各个阶段引起的卵泡变化对于进一步了解临床使用这些组织保存生育能力的安全性和有效性至关重要。我们的研究首次分析了从早期卵泡中收集的单个新鲜和慢速冷冻/解冻的人类卵母细胞之间的转录组变化。为了实现这一目标，我们开发了一种分离新鲜和冷冻/解冻的人类卵巢皮层的新方法，以获得来自早期卵泡的活剥卵母细胞。我们的研究结果为使用冷冻保存组织和卵泡来保存生育能力提供了见解。研究资金/竞争利益：本工作由美国国立卫生研究院（NIH） R01HD099402，生殖生物学职业培训（CTRB）培训资助美国国立卫生研究院（NIH） T32给Jordan Machlin，美国国立卫生研究院（NIH） F31-HD106626和美国国立卫生研究院（NIH） T31H-D079342给Andrea Jones，美国国立卫生研究院（NIH） T32- gm70449给D. Ford Hannum，以及Chan Zuckerberg Initiative Grant CZF2019-002428资助。我们没有利益冲突要申报。

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来源期刊

Human reproduction 医学-妇产科学

CiteScore

10.90

自引率

6.60%

发文量

1369

审稿时长

1 months

期刊介绍： Human Reproduction features full-length, peer-reviewed papers reporting original research, concise clinical case reports, as well as opinions and debates on topical issues. Papers published cover the clinical science and medical aspects of reproductive physiology, pathology and endocrinology; including andrology, gonad function, gametogenesis, fertilization, embryo development, implantation, early pregnancy, genetics, genetic diagnosis, oncology, infectious disease, surgery, contraception, infertility treatment, psychology, ethics and social issues.