Background
It has been decades since the first in vitro fertilization (IVF) infant was born; since then, assisted reproduction has advanced significantly. The number of available embryos in each IVF cycle has also increased, resulting in a slew of surplus of embryos undergoing cryopreservation. Cryopreservation of embryos increases the cumulative pregnancy rate for a single cycle of ovarian stimulation with the clinical pregnancy rate and live birth rate being no lower than in the fresh cycle, while reducing the risk of multiple pregnancies and ovarian stimulation [
1‐
3]. As such, cryopreservation has become a widespread reliable procedure in assisted reproductive technologies [
4]. However, many studies have also shown that frozen-thawed embryo transfer (FET) increases the risks of pregnancy-induced hypertension, large for gestational age and high birth weight infants compared with fresh embryo transfer [
5‐
7].
With the implementation of the single embryo transfer strategy, the number of surplus embryos has increased [
8]. When more than one embryo was frozen in one cryo-straw but only one embryo was transferred, the surplus embryo will be refrozen. Dose re-cryopreservation have negative effects on clinical outcomes? On present understanding, repeated cryopreservation procedures may reduce embryo implantation rate,clinical pregnancy rate and live birth rate [
9,
10]. However, limited published data have focused on the perinatal outcomes of embryos experiencing repeated cryopreservation. Due to heterogeneity between studies, the current conclusions are not clear. Therefore, in order to further clarify whether repeated cryopreservation has adverse effects on offspring, we retrospectively analyzed the perinatal outcome of embryos repeated cryopreservation by vitrification in the present study.
Methods
Study design
This retrospective study was approved by the Medical Ethics Committee of Nanjing Drum Tower Hospital affiliated to Nanjing University Medical School on 6 May 2021 (reference number 2021–163-01).
All medical files including frozen-thawed blastocyst cycles from January 2013 to December 2019 at the Reproductive Medicine Centre of Nanjing Drum Tower Hospital were retrospectively reviewed. Inclusion criteria: (1) patients undergoing single blastocyst transfer with live singleton births and known perinatal outcomes; (2) patients have experienced at least one frozen-thawed cycle and did not have a live birth in the preceding cycle. Patients with endometriosis, abnormal uterine pathology or undergoing preimplantation genetic testing or those with history of recurrent pregnancy loss were excluded. In total, 647 live born singletons were included in this study. They were divided into two groups according to the transferred embryo cryopreservation time: vitrified-warmed blastocysts (once-vitrified group, n = 592) and vitrified-warmed blastocysts derived from thawed cleaved embryos (re-vitrified group, n = 55).
IVF/ICSI procedure and embryo culture
Depending on the patient’s age, ovarian reserve, and ovarian responses in the previous ovulation cycle, gonadotrophin-releasing hormone (GnRH) agonist protocol or antagonist protocol was used [
11].
GnRH-agonist protocol: In mid luteal phase of the preceding cycle, a short-acting GnRH-a (Triptorelin, Ferring AG, Germany) was administered daily for 14 days and follicular ultrasonography, serum luteinizing hormone (LH), follicle stimulating hormone (FSH), estradiol (E2) and progesterone were measured. 150–300 IU recombinant FSH (Gonal-F, Merck Serono, Switzerland) was administered daily when the serum FSH and LH levels were < 5 mIU/mL and E2 was < 50 pg/mL. GnRH-a was continued until the trigger day. The dosage of recombinant FSH was adjusted according to the ovarian response, and human menopausal gonadotropin (HMG, LIVZON, China) or recombinant LH (Luveris, Merck Serono, Switzerland) was added as needed.
GnRH-antagonist protocol: 150–300 IU recombinant FSH was initiated on Day 2 or 3 of the menstrual cycle until trigger day. The dosage of recombinant FSH was adjusted, and HMG or recombinant LH was added according to the ovarian response evaluated by transvaginal ultrasonography and serum hormone levels. 0.25 mg cetrorelix (Cetrotide, Merck Serono, France) was used daily when the leading follicles reached a mean diameter of 14 mm until trigger day.
For both protocols, if two to three dominant follicles reached a diameter of 18 mm, 250 μg recombinant human chorionic gonadotropin (hCG) (Ovitrelle, Merck Serono, France) was injected. The oocytes were retrieved under transvaginal ultrasound guidance 36–38 hours after recombinant hCG administration. Retrieved oocytes were then fertilized in conventional IVF or intracytoplasmic sperm injection (ICSI). Two pronuclei or two polar bodies can be observed in normal fertilization 16–18 h post insemination. Embryos were cultured in G1/G2 sequential media (Vitrolife, Goteborg, Sweden) at 37 °C in 6% CO
2, 5% O
2 and 89% N
2 high-humidity incubator. Blastocyst morphological evaluation was based on the Gardner scoring system [
12].
Vitrification cryopreservation and thawing procedures
The vitrification cryopreservation and thawing procedures were carried out using a vitrification or warming kit from Kitazato (Tokyo, Japan). Before vitrification, the blastocyst was artificially shrunken by laser drilling. Cleavage-stage embryos or shrunken blastocysts were preequilibrated in equilibration solution for 5–8 min at room temperature and then placed into vitrification solution. One minute later, the embryos were loaded onto the surface of Cryotop (Kitazato, Tokyo, Japan) and then submerged into liquid nitrogen immediately, using open vitrification devices.
The warming procedure was referred to our center’s previous research [
13]. The embryo was immediately transferred to preequilibrated thawing solution for 1 min and dilution solution for 3 min and then washed twice in washing solutions 1 and 2 for 5 min each; the embryo was then cultured in a 100 μl droplet of culture medium G2 (Vitrolife, Goteborg, Sweden) overlaid with light paraffin oil (Vitrolife, Goteborg, Sweden) in the incubator at 37 °C in a humidified atmosphere with 5% O
2, 6% CO
2 and 89% N
2 for 2–4 h and then assessed. Laser-assisted hatching was applied to vitrified–warmed blastocysts except for those blastocysts with an expansion degree of V or VI. Generally, blastocysts with re-expanded blastocoel cavities with clear morphology and a bright lustre were considered to have survived.
Outcome measures
Overall baseline clinical characteristics for each patient included age, body mass index (BMI), basal FSH, duration of infertility, parity, type of infertility and cause of infertility, insemination methods (IVF or ICSI), endometrium preparation protocol for FET, and endometrial thickness.
Any singleton birth ≥24 weeks of gestation was considered a live singleton birth. The birth weight, gestational age at delivery and sex were recorded for all live singletons. The neonatal outcomes evaluated were preterm birth (PTB, delivery between 24 and 37 weeks), low birthweight (LBW, birthweight < 2500 g), macrosomia (birthweight > 4000 g), average birthweight, sex ratio, small for gestational age (SGA), and large for gestational age (LGA). SGA was defined as a weight below the 10th percentile for gestational age, and LGA was defined as having a birthweight greater than the 90th percentile for gestational age at birth [
14].
Statistical analysis
Continuous variables were described by using the mean ± SD or median (interquartile range, IQR), while categorical variables were described as absolute numbers and percentages. Student’s test was used to compare the differences of normally distribution parameters, while for non-normal distribution parameters, Wilcoxon rank sum test were used. Pearson’s chi-squared test or Fisher’s precision probability test was used to compare the differences of categorical variables. To help account for the nonrandomized administration of re-vitrified embryos, we used propensity-score methods to reduce the effects of confounding. Matching was performed with the use of a 1:1 matching protocol without replacement, with a caliper width equal to 0.01 of the standard deviation of the logit of the propensity score. P values < 0.05 were considered statistically significant. The variables included maternal age, parity, basal FSH, BMI, duration of infertility, type of infertility, parity, and cause of infertility. To analyse the associations between the cryopreserved time and perinatal outcomes, logistic regression models were conducted for each outcome indicator using the before and after matching data, and odds ratios (OR) and their 95% CI before and after adjusting for confounders were calculated. Statistical analyses were performed using SPSS statistical package version 26.0.
Discussion
More and more children are born using assisted reproductive technology (ART) globally, so the safety of offspring is increasingly concerned. In this retrospective study, we assessed the effect of repeated vitrification-warming procedures on perinatal outcomes of human embryos. According to our research results, no poor outcomes were observed among singletons following repeated vitrification-warming procedures compared to once vitrification-warming procedures.
Embryo cryopreservation is a crucial part of ART. Compared with fresh embryo transfer, frozen embryo transfer is associated with a higher risk of LGA and higher birth weight in singletons [
6,
15]. However, the safety of offspring after repeated frozen embryo transfer has not been widely reported at present. After all, re-cryopreservation of embryos is an occasional event. There were several case reports demonstrating healthy live births after frozen-thawed embryo transfer cycles with embryos that were frozen-thawed twice [
16‐
18]. And some early retrospective studies have also shown that the embryos re-cryopreservation does not affect clinical pregnancy rates [
19,
20]. However, other recent studies have shown that transfer of twice frozen-thawed embryos increase the rate of miscarriage and reduce the clinical pregnancy rate and live birth rate [
9,
10,
21]. The discrepancies in the results of these studies may be due to the different methods used to freeze embryos,embryos frozen at different stages and the differences in baseline characteristics of the study population. Furthermore, these studies may exist the sample selection biases, as the patients underwent repeated cryopreserved embryo transfer may always experience previous embryo transfer failure, so the control group should be consistent with this. The first follow-up study to present perinatal outcomes of children born after embryo re-cryopreservation showed that human refrozen-thawed embryos resulted in normal live births after FET at a similar rate to that of once-frozen-thawed embryos [
22]; however, detailed neonatal outcomes were not described. Two other studies reported that repeated cryopreservation of embryos have no negative impact on neonatal outcomes [
9,
21], but they did not eliminate the possible bias of confounding factors on the results.
In the present study, patients who had experienced previous embryo transfer failure were set as the once-vitrified group, and all embryos were frozen using the same vitrification method. Furthermore, to eliminate the influence of clinical baseline characteristics on the results, a propensity score matching, and logistic regression were used to control for potential confounding variables. After PSM, the incidence of PTB, LBW, macrosomia and LGA was not different between the once-vitrified group and the re-vitrified group. Logistic regression after adjusting for relevant confounding factors showed that the number of vitrification-warming procedures was not related to the incidence of PTB, LBW, macrosomia, LGA or birthweight.
It has been reported that the effect of FET on birthweight may interact with sex [
7,
23]. Litzky et al.’s study indicated that FET influenced male birthweight, but it did not have effects on female birthweight [
7]. To eliminate this important confounder, we performed sex-stratified analyses to improve interpretability in our study. There was no significant difference in birthweight, LBW, or macrosomia in either male or female neonates. In addition, perinatal outcomes are also closely related to maternal obstetric complications. For singletons, the risk of hypertensive disorders after FET was higher than after fresh cycles or spontaneous pregnancies [
24,
25]. The increased risk of hypertensive disorders among FET may be related to alteration in methylation of regulatory genes involved with implantation or to programmed FET protocols [
26,
27]. Whereas the association of FET with GDM is deficient in previous studies [
28‐
30]. Studies have shown that hypertensive disorders of pregnancy increase the prevalence of low birth weight [
31], and gestational diabetes mellitus (GDM) increases the incidence of macrosomia [
32,
33]. Consequently, we further analysed maternal complications in the once-vitrified group and re-vitrified group. There was no difference in gestational hypertension or gestational diabetes before and after data matching. Also, other maternal complications did not differ between the two groups, as shown in Supplemental Table
1. Therefore, the bias caused by maternal complications during pregnancy can be excluded.
Of course, there are several limitations in our study. First, it was a retrospective study with single-centre participation. Second, although we used propensity score matching to eliminate the influence of baseline characteristics on FET outcomes as much as possible, it could not eliminate all bias caused by confounders between the two groups. In addition, because of the limited sample size, it was difficult to stratify the effects of repeated vitrification-warming procedures on birthweight by gestational age. And some indicators of newborns (such as APGAR scores and NICU rate) were not included in our follow-up database, which needs to be improved in the future. Moreover, some meaningful variables (such as the duration of embryo cryopreservation and perinatal outcomes of fresh embryo transfer cycles) were not included in this study, which may also create a bias. Nevertheless, the present study still presented perinatal outcomes of singletons following double vitrification-warming procedures, which are occasional in the clinic, providing valuable information for clinical decision-making.
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