Your search keyword '"Tan, Yue-Qiu"' showing total 13 results

1. Next-generation sequence-based preimplantation genetic testing for monogenic disease resulting from maternal mosaicism.

Author

Hu X, He WB, Zhang SP, Luo KL, Gong F, Dai J, Zhang Y, Wan ZX, Li W, Yuan SM, Tan YQ, Lu GX, Lin G, and Du J

Subjects

Adult, Blastocyst metabolism, Female, Genetic Diseases, Inborn diagnosis, High-Throughput Nucleotide Sequencing methods, Humans, Male, Mutation, Sequence Analysis, DNA methods, Genetic Diseases, Inborn genetics, Genetic Testing methods, Mosaicism, Preimplantation Diagnosis methods

Abstract

Background: Mosaicism poses challenges for genetic counseling and preimplantation genetic testing for monogenic disorders (PGT-M). NGS-based PGT-M has been extensively used to prevent the transmission of monogenic defects, but it has not been evaluated in the application of PGT-M resulting from mosaicism., Methods: Four women suspected of mosaicism were confirmed by ultra-deep sequencing. Blastocyst trophectoderm cells and polar bodies were collected for whole genome amplification, followed by pathogenic variants detection and haplotype analysis based on NGS. The embryos free of the monogenic disorders were transplantable., Results: Ultra-deep sequencing confirmed that the four women harbored somatic mosaic variants, with the proportion of variant cells at 1.12%, 9.0%, 27.60%, and 91.03%, respectively. A total of 25 blastocysts were biopsied and detected during four PGT cycles and 5 polar bodies were involved in one cycle additionally. For each couple, a wild-type embryo was successfully transplanted and confirmed by prenatal diagnosis, resulting in the birth of four healthy infants., Conclusions: Mosaic variants could be effectively evaluated via ultra-deep sequencing, and could be prevented the transmission by PGT. Our work suggested that an NGS-based PGT approach, involving pathogenic variants detection combined with haplotype analysis, is crucial for accurate PGT-M with mosaicism., (© 2021 The Authors. Molecular Genetics & Genomic Medicine published by Wiley Periodicals LLC.)

Published

2021

2. Clinical outcomes following preimplantation genetic testing and microdissecting junction region in couples with balanced chromosome rearrangement.

Author

Cheng D, Hu L, Gong F, Yuan S, Luo K, Wu X, Xie P, Lu C, Lu G, Tan YQ, and Lin G

Subjects

Adult, Chromosome Disorders genetics, Embryo Transfer, Female, Humans, Male, Pregnancy, Pregnancy Outcome, Pregnancy Rate, Retrospective Studies, Chromosome Aberrations statistics & numerical data, Chromosome Disorders diagnosis, Fertilization in Vitro methods, Genetic Testing methods, Preimplantation Diagnosis methods

Abstract

Purpose: The purpose of this study is to summarize the clinical outcomes of apparently balanced chromosome rearrangement (ABCR) carriers in preimplantation genetic testing (PGT) cycles by next-generation sequencing following microdissecting junction region (MicroSeq) to distinguish non-carrier embryos from balanced carriers., Methods: A retrospective study of 762 ABCR carrier couples who requested PGT for structural rearrangements combined with MicroSeq at the Reproductive and Genetic Hospital of CITIC-Xiangya was conducted between October 2014 and October 2019., Results: Trophectoderm biopsy was performed in 4122 blastocysts derived from 917 PGT-SR cycles and 3781 blastocysts were detected. Among the 3781 blastocysts diagnosed, 1433 (37.9%, 1433/3781) were balanced, of which 739 blastocysts were carriers (51.57%, 739/1433) and 694 blastocysts were normal (48.43%, 694/1433). Approximately 26.39% of cycles had both carrier and normal embryo transfer, and the average number of biopsied blastocysts was 6.7. In the cumulative 223 biopsied cycles with normal embryo transfer, all couples chose to transfer the normal embryos. In the 225 cycles with only carrier embryos, the couples chose to transfer the carrier embryos in 169/225 (75.11%) cycles. A total of 732 frozen embryo transfer cycles were performed, resulting in 502 clinical pregnancies. Cumulatively, 326 babies were born; all of these babies were healthy and free of any developmental issues., Conclusion: Our study provides the first evaluation of the clinical outcomes of a large sample with ABCR carrier couples undergoing the MicroSeq-PGT technique and reveals its powerful ability to distinguish between carrier and non-carrier balanced embryos.

Published

2021

3. Analysis of molecular cytogenetic features and PGT-SR for two infertile patients with small supernumerary marker chromosomes.

Author

Cheng D, Yuan S, Yi D, Luo K, Xu F, Gong F, Lu C, Lu G, Lin G, and Tan YQ

Subjects

Adult, Chromosomes genetics, Chromosomes, Human, Pair 3 genetics, Female, High-Throughput Nucleotide Sequencing, Humans, Infertility genetics, Infertility pathology, Karyotype, Karyotyping, Male, Mosaicism, Trisomy pathology, Chromosome Aberrations, Cytogenetic Analysis, Genetic Testing, Trisomy genetics

Abstract

Research Question: Can preimplantation genetic testing for structural rearrangement (PGT-SR) with next-generation sequencing (NGS) be used to infertile patients carrying small supernumerary marker chromosomes (sSMCs)?, Design: In this study, two infertile patients carrying ring sSMCs were recruited. Different molecular cytogenetic techniques were performed to identify the features of the two sSMCs, followed by clinical PGT-SR cycles., Results: The results of G-banding and FISH showed that patient 1's sSMC originated from the 8p23-p10 region, with a resulting karyotype of [ 47,XY, del(8)(p23p10), +r(8)(p23p10).ish del(8)(CEP8+,subtle 8p+,subtle 8q+),r(8)(CEP8+,subtle 8p-,subtle 8q-)[55/60].arr(1-22) ×2,(X,Y)×1]. The sSMC of patient 2 was derived from chromosome 3 and further microdissection with next-generation sequencing (MicroSeq) revealed it contained the region of chromosome 3 between 93,504,855 and 103,839,892 bp (GRCh37), which involved 52 known genes. So the karyotype of patient 2 was 47,XX, +mar.ish der(3)(CEP3+,subtle 3p-,subtle 3q-)[49/60].arr[GRCh37] 3q11.2q13.1(93,500,001_103,839,892) ×3(0.5). PGT-SR with NGS was performed to provide reproductive guidance for the two patients. For patient 1, four balanced euploid embryos and four embryos with partial trisomy/monosomy of (8p23.1-8p11.21) were obtained, and a balanced euploid embryo was successfully implanted and had resulted in a healthy baby. For patient 2, an embryo with monosomy of sex chromosomes and another embryo with a duplication at (3q11-q13.1), neither of which was available for implantation., Conclusions: The identification of the origins and structural characteristics of rare sSMCs should rely on different molecular cytogenetic techniques. PGT-SR is an alternative fertility treatment for these patients carrying sSMCs. This study may provide directions for the assisted reproductive therapy for infertile patients with sSMC.

Published

2019

4. Neonatal outcomes of live births after blastocyst biopsy in preimplantation genetic testing cycles: a follow-up of 1,721 children.

Author

He H, Jing S, Lu CF, Tan YQ, Luo KL, Zhang SP, Gong F, Lu GX, and Lin G

Subjects

Adult, Biopsy adverse effects, Birth Weight, Female, Gestational Age, Humans, In Situ Hybridization, Fluorescence, Infant, Low Birth Weight, Infant, Newborn, Infant, Premature, Live Birth, Predictive Value of Tests, Pregnancy, Premature Birth etiology, Retrospective Studies, Risk Assessment, Risk Factors, Sperm Injections, Intracytoplasmic, Treatment Outcome, Blastocyst pathology, Embryo Transfer adverse effects, Fertilization in Vitro adverse effects, Genetic Testing, Preimplantation Diagnosis methods

Abstract

Objective: To investigate whether blastocyst biopsy in preimplantation genetic testing (PGT) increases the risk of adverse neonatal outcomes., Design: Retrospective cohort study., Setting: University-affiliated center., Patients: Live births after blastocyst biopsy combined with frozen ET (PGT group) and frozen blastocyst transfer after in vitro fertilization or intracytoplasmic sperm injection (control group)., Intervention(s): Blastocyst biopsy., Main Outcome Measure(s): Gestational age (GA), birth weight (BW), and rates of preterm birth (PB), very preterm birth (VPB), extreme preterm birth (EPB), low birth weight (LBW), very low birth weight (VLBW), and macrosomia., Result(s): No significant differences were observed in the sex ratio, GA, PB, VPB, EPB, BW, or rates of LBW, VLBW, and macrosomia between the PGT and control groups for either singletons or twins. However, the cesarean section rate of the PGT group was significantly higher than that of the control group for twins (adjusted odds ratio, 2.383 [1.079, 5.259]). Regarding fluorescence in situ hybridization-PGT neonates, neonatal outcomes, including GA, BW, and rates of PB, VPB, LBW, and VLBW, did not differ between the different groups of biopsied cells (≥10 group and <10 group) for either the grade B or grade C trophectoderm score subgroups; however, in the grade B trophectoderm score subgroup, the rate of boy babies in the ≥10 group was significantly higher than that in the <10 group (83.3% vs. 40.9%). The association between the number of biopsied cells and GA/BW was not statistically significant., Conclusion(s): Blastocyst biopsy may not add additional risk to neonatal outcomes when compared with a control group., (Copyright © 2019 American Society for Reproductive Medicine. Published by Elsevier Inc. All rights reserved.)

Published

2019

5. Expanded carrier screening and preimplantation genetic diagnosis in a couple who delivered a baby affected with congenital factor VII deficiency.

Author

He WB, Tan YQ, Hu X, Li W, Xiong B, Luo KL, Gong F, Lu GX, Lin G, and Du J

Subjects

Aneuploidy, Cystic Fibrosis diagnosis, Cystic Fibrosis genetics, Cystic Fibrosis prevention & control, Factor VII genetics, Factor VII metabolism, Factor VII Deficiency prevention & control, Female, Fertilization in Vitro, Gene Deletion, Genes, Recessive, Genetic Diseases, Inborn diagnosis, Genetic Diseases, Inborn genetics, Genetic Diseases, Inborn prevention & control, Genetic Predisposition to Disease, Humans, Infant, Male, Pedigree, Pregnancy, Pregnancy Outcome, Sequence Analysis, DNA, Whole Genome Sequencing, Cystic Fibrosis Transmembrane Conductance Regulator genetics, Factor VII Deficiency diagnosis, Factor VII Deficiency genetics, Genetic Testing, Preimplantation Diagnosis

Abstract

Background: Preimplantation genetic diagnosis (PGD) is a powerful tool for preventing the transmission of Mendelian disorders from generation to generation. However, PGD only can identify monogenically inherited diseases, but not other potential monogenic pathologies. We aimed to use PGD to deliver a healthy baby without congenital FVII deficiency or other common Mendelian diseases in a couple in which both individuals carried a deleterious mutation in the F7 gene., Methods: After both members of the couple were confirmed to be carriers of the F7 gene mutation by Sanger sequencing, expanded carrier screening (ECS) for 623 recessive inheritance diseases was performed to detect pathological mutations in other genes. PGD and preimplantational genetic screening (PGS) were employed to exclude monogenic disorders and aneuploidy for their embryos., Results: ECS using targeted capture sequencing technology revealed that the couple carried the heterozygous disease-causative mutations c.3659C > T (p.Thr1220Ile) and c.3209G > A (p.Arg1070Gln) in the CFTR gene. After PGD and PGS, one of their embryos that was free of congenital FVII deficiency, cystic fibrosis (CF) and aneuploidy was transferred, resulting in the birth of a healthy 3200 g male infant., Conclusion: We successfully implemented PGD for congenital FVII deficiency and PGD after ECS to exclude CF for the first time to the best of our knowledge. Our work significantly improved the reproductive outcome for the couple and provides a clear example of the use of ECS combined with PGD to avoid the delivery of offspring affected not only by identified monogenically inherited diseases but also by other potential monogenic pathologies and aneuploidy.

Published

2018

6. Extended application of PGT-M strategies for small pathogenic CNVs.

Author

Hu, Xiao, Wang, Weili, Luo, Keli, Dai, Jing, Zhang, Yi, Wan, Zhenxing, He, Wenbin, Zhang, Shuoping, Yang, Lanlin, Tan, Qin, Li, Wen, Zhang, Qianjun, Gong, Fei, Lu, Guangxiu, Tan, Yue-Qiu, Lin, Ge, and Du, Juan

Subjects

WHOLE genome sequencing, GENETIC testing, HAPLOTYPES, PRENATAL diagnosis, AMNIOTIC liquid, CHROMOSOMES, PREGNANCY

Abstract

Purpose: The preimplantation genetic testing for aneuploidy (PGT-A) platform is not currently available for small copy-number variants (CNVs), especially those < 1 Mb. Through strategies used in PGT for monogenic disease (PGT-M), this study intended to perform PGT for families with small pathogenic CNVs. Methods: Couples who carried small pathogenic CNVs and underwent PGT at the Reproductive and Genetic Hospital of CITIC-Xiangya (Hunan, China) between November 2019 and April 2023 were included in this study. Haplotype analysis was performed through two platforms (targeted sequencing and whole-genome arrays) to identify the unaffected embryos, which were subjected to transplantation. Prenatal diagnosis using amniotic fluid was performed during 18–20 weeks of pregnancy. Results: PGT was successfully performed for 20 small CNVs (15 microdeletions and 5 microduplications) in 20 families. These CNVs distributed on chromosomes 1, 2, 6, 7, 13, 15, 16, and X with sizes ranging from 57 to 2120 kb. Three haplotyping-based PGT-M strategies were applied. A total of 89 embryos were identified in 25 PGT cycles for the 20 families. The diagnostic yield was 98.9% (88/89). Nineteen transfers were performed for 17 women, resulting in a 78.9% (15/19) clinical pregnancy rate after each transplantation. Of the nine women who had healthy babies, eight accepted prenatal diagnosis and the results showed no related pathogenic CNVs. Conclusion: Our results show that the extended haplotyping-based PGT-M strategy application for small pathogenic CNVs compensated for the insufficient resolution of PGT-A. These three PGT-M strategies could be applied to couples with small pathogenic CNVs. [ABSTRACT FROM AUTHOR]

Published

2024

7. Non-invasive preimplantation genetic testing for conventional IVF blastocysts.

Author

Xie, Pingyuan, Zhang, Shuoping, Gu, Yifang, Jiang, Bo, Hu, Liang, Tan, Yue-qiu, Yao, Yaxin, Tang, Yi, Wan, Anqi, Cai, Sufen, Zou, Yangyun, Lu, Guangxiu, Wan, Cheng, Gong, Fei, Lu, Sijia, and Lin, Ge

Subjects

INTRACYTOPLASMIC sperm injection, FERTILIZATION in vitro, GENETIC testing, BLASTOCYST, POLYPLOIDY, GENE amplification, CULTURE media (Biology), SEMEN, PREIMPLANTATION genetic diagnosis, CHROMOSOME abnormalities, RESEARCH funding

Abstract

Background: Previous studies suggested that non-invasive preimplantation genetic testing (niPGT) for intracytoplasmic sperm injection (ICSI) blastocysts can be used to identify chromosomal ploidy and chromosomal abnormalities. Here, we report the feasibility and performance of niPGT for conventional in vitro fertilization (IVF) blastocysts.Methods: This was a prospective observational study. In the preclinical stage, whole genome amplification and NGS were performed using the sperm spent culture medium (SCM). Then, trophectoderm (TE) biopsies and corresponding SCM derived from 27 conventional IVF monopronuclear embryos were collected. In the clinical stage, samples from 25 conventional IVF cycles and 37 ICSI cycles from April 2020-August 2021 were collected for performance evaluation.Results: Preclinically, we confirmed failed sperm DNA amplification under the current amplification system. Subsequent niPGT from the 27 monopronuclear blastocysts showed 69.2% concordance with PGT results of corresponding TE biopsies. In the clinical stage, no paternal contamination was observed in any of the 161 SCM samples from conventional IVF. While maternal contamination was observed in 29.8% (48/161) SCM samples, only 2.5% (4/161) samples had a contamination ratio ≥ 50%. Compared with that of TE biopsy, the performances of NiPGT from 161 conventional IVF embryos and 122 ICSI embryos were not significantly different (P > 0.05), with ploidy concordance rates of 75% and 74.6% for IVF and ICSI methods, respectively. Finally, evaluation of the euploid probability of embryos with different types of niPGT results showed prediction probabilities of 82.8%, 77.8%, 62.5%, 50.0%, 40.9% and 18.4% for euploidy, sex-chromosome mosaics only, low-level mosaics, multiple abnormal chromosomes, high-level mosaics and aneuploidy, respectively.Conclusions: Our research results preliminarily confirm that the niPGT approach using SCM from conventional IVF has comparable performance with ICSI and might broadening the application scope of niPGT. [ABSTRACT FROM AUTHOR]

Published

2022

8. Risk Factors Affecting Alternate Segregation in Blastocysts From Preimplantation Genetic Testing Cycles of Autosomal Reciprocal Translocations.

Author

Xie, Pingyuan, Hu, Liang, Peng, Yangqin, Tan, Yue-qiu, Luo, Keli, Gong, Fei, Lu, Guangxiu, and Lin, Ge

Subjects

GENETIC testing, CHROMOSOMAL rearrangement, GENETIC counseling

Abstract

Reciprocal translocations are the most common structural chromosome rearrangements and may be associated with reproductive problems. Therefore, the objective of this study was to analyze factors that can influence meiotic segregation patterns in blastocysts for reciprocal translocation carriers. Segregation patterns of quadrivalents in 10,846 blastocysts from 2,871 preimplantation genetic testing cycles of reciprocal translocation carriers were analyzed. The percentage of normal/balanced blastocysts was 34.3%, and 2:2 segregation was observed in 90.0% of the blastocysts. Increased TAR1 (ratio of translocated segment 1 over the chromosome arm) emerged as an independent protective factor associated with an increase in alternate segregation (p = 0.004). Female sex and involvement of an acrocentric chromosome (Acr-ch) were independent risk factors that reduced alternate segregation proportions (p < 0.001). Notably, a higher TAR1 reduced the proportion of adjacent-1 segregation (p < 0.001); a longer translocated segment and female sex increased the risk of adjacent-2 segregation (p = 0.009 and p < 0.001, respectively). Female sex and involvement of an Acr-ch enhanced the ratio of 3:1 segregation (p < 0.001 and p = 0.012, respectively). In conclusion, autosomal reciprocal translocation carriers have reduced proportions of alternate segregation in blastocysts upon the involvement of an Acr-ch, female sex, and lower TAR1. These results may facilitate more appropriate genetic counseling for couples with autosomal reciprocal translocation regarding their chances of producing normal/balanced blastocysts. [ABSTRACT FROM AUTHOR]

Published

2022

9. The genetic cause of intellectual deficiency and/or congenital malformations in two parental reciprocal translocation carriers and implications for assisted reproduction.

Author

Cheng, Dehua, Yuan, Shimin, Hu, Liang, Yi, Duo, Luo, Keli, Gong, Fei, Lu, Changfu, Lu, Guangxiu, Lin, Ge, and Tan, Yue-Qiu

Subjects

CHROMOSOMAL translocation, REPRODUCTIVE technology, HUMAN abnormalities, GENETIC testing, HUMAN chromosome abnormality diagnosis, GENETIC counseling, HUMAN artificial insemination, HUMAN embryo transfer

Abstract

Purpose: To elucidate the genetic cause of intellectual deficiency and/or congenital malformations in two parental reciprocal translocation carriers and provide appropriate strategies of assisted reproductive therapy (ART). Materials and methods: Two similar couples having a child with global developmental delay/intellectual disability symptoms attended the Reproductive and Genetic Hospital of CITIC-Xiangya (Changsha, China) in 2017 and 2019, respectively, in order to determine the cause(s) of the conditions affecting their child and to seek ART to have a healthy baby. Both of the healthy couples were not of consanguineous marriage, denied exposure to toxicants, and had no adverse life history. This study was approved by the Institutional Ethics Committee of the Reproductive & Genetic Hospital of CITIC-Xiangya, and written informed consent was obtained from the parents. Genetic diagnoses were performed by karyotype analysis, breakpoint mapping analysis of chromosomal translocation(s), single-nucleotide polymorphism (SNP) microarray analysis, and whole-exome sequencing (WES) for the two children and different appropriate reproductive strategies were performed in the two families. Results: Karyotype analysis revealed that both patients carried parental reciprocal translocations [46,XY,t(7;16)(p13;q24)pat and 46,XY,t(13;17)(q12.3;p11.2)pat, respectively]. Follow-up breakpoint mapping analysis showed no interruption of associated genes, and SNP microarray analysis identified no significant copy number variations (CNVs) in the two patients. Moreover, WES results revealed that patients 1 and 2 harbored candidate compound heterozygous mutations of MCOLN1 [c.195G>C (p.K65N) and c.1061G>A (p.W354*)] and MCPH1 [c.877A>G (p.S293G) and c.1869_1870delAT (p.C624*)], respectively, that were inherited from their parents and not previously reported. Furthermore, the parents of patient 1 obtained 10 embryos during ART cycle, and an embryo of normal karyotype and non-carrier of observed MCOLN1 mutations according to preimplantation genetic testing for structural rearrangement and monogenic defect was successfully transferred, resulting in the birth of a healthy boy. The parents of patient 2 chose to undergo ART with donor sperm to reduce the risk of recurrence. Conclusions: Systematic genetic diagnosis of two carriers of inherited chromosomal translocations accompanied by clinical phenotypes revealed their cause of disease, which was critical for genetic counseling and further ART for these families. [ABSTRACT FROM AUTHOR]

Published

2021

10. Breakpoint mapping uncovering about 1.32% of apparent balanced reciprocal translocation (ABRT) carriers existing cryptic complex chromosomal structural variations in preimplantation genetic testing (PGT).

Author

Yuan, Shimin and Tan, Yue-qiu

Subjects

*GENETIC testing, *GENETIC variation

Published

2019

11. Novel variants of the PCCB gene in Chinese patients with propionic acidemia.

Author

Yang, Xiaoxuan, Li, Dongyan, Tu, Chaofeng, He, Wenbing, Meng, Lanlan, Tan, Yue-Qiu, Lu, Guangxiu, Du, Juan, and Zhang, Qianjun

Subjects

*CHINESE people, *ACIDOSIS, *EMBRYO implantation, *FERTILIZATION in vitro, *GENETIC testing, *HUMAN in vitro fertilization, *RECESSIVE genes

Abstract

• We analyzed clinical characteristics of four individuals with propionic acidemia. • Through whole-exome sequencing and SNP-array, five PCCB variants were identified. • Preimplantation genetic testing guided the successful embryo transfer and implantation. Propionic acidemia (PA) is an autosomal recessive metabolic disorder caused by a deficiency of propionyl-CoA carboxylase and mutations in the PCCA and PCCB genes. In this study, we investigated the clinical characteristics of individuals with PA and conducted genetic analyses to provide new genetic evidence for the diagnosis of PA. We conducted whole-exome sequencing and Sanger sequencing in four individuals with PA from three unrelated Chinese families. We also performed a structural analysis of the PCCB protein variants. Couples from the three families included in our study underwent in vitro fertilization with preimplantation genetic testing. We found five variants of PCCB. These biallelic variants were inherited from heterozygous parental carriers and were located in the functional domain, absent in human population genome datasets, and predicted to be deleterious. These findings indicate that the variants might be responsible for the clinical features observed in these particular patients with PA. Through successful embryo transfer and implantation, one of the couples fortunately gave birth to a healthy child. Overall, our study can expand the mutation spectrum of PCCB and provide useful information for the prenatal diagnosis of PA and genetic counseling for affected individuals. [ABSTRACT FROM AUTHOR]

Published

2021

12. Reproductive risks and preimplantation genetic testing intervention for X–autosome translocation carriers.

Author

Yuan, Shimin, Cheng, Dehua, Luo, Keli, Li, Xiurong, Hu, Liang, Hu, Hao, Wu, Xianhong, Xie, Pingyuan, Lu, Changfu, Lu, Guangxiu, Lin, Ge, Gong, Fei, and Tan, Yue-Qiu

Subjects

*GENETIC engineering, *GENETIC testing, *CONGENITAL heart disease, *X chromosome, *EMBRYO transfer, *MULTIPLE pregnancy, *SYNOVIOMA

Abstract

What is the genetic cause of multiple congenital disabilities in a girl with a maternal balanced X–autosome translocation [t(X-A)]? Is preimplantation genetic testing (PGT), to distinguish non-carrier from euploid/balanced embryos and prioritize transfer, an effective and applicable strategy for couples with t(X-A)? Karyotype analysis, whole-exome sequencing and X inactivation analysis were performed for a girl with congenital cardiac anomalies, language impairment and mild neurodevelopmental delay. PGT based on next-generation sequencing after microdissecting junction region (MicroSeq) to distinguish non-carrier and carrier embryos was used in three couples with a female t(X-A) carrier (cases 1–3). The girl carried a maternal balanced translocation 46,X,t(X;1)(q28;p31.1). Whole-exome sequencing revealed no monogenic mutation related to her phenotype, but she carried a rare skewed inactivation of the translocated X chromosome that spread to the adjacent interstitial 1p segment, contrary to her mother. All translocation breakpoints in cases 1–3 were successfully identified and each couple underwent one PGT cycle. Thirty oocytes were retrieved, and 13 blastocysts were eligible for biopsy, of which six embryos had a balanced translocation and only four were non-carriers. Three cryopreserved embryo transfers with non-carrier status embryos resulted in the birth of two healthy children (one girl and one boy), who were subsequently confirmed to have normal karyotypes. This study reported a girl with multiple congenital disabilities associated with a maternal balanced t(X-A) and verified that the distinction between non-carrier and carrier embryos is an effective and applicable strategy to avoid transferring genetic and reproductive risks to the offspring of t(X-A) carriers. [ABSTRACT FROM AUTHOR]

Published

2021

13. A homozygous RPL10L missense mutation associated with male factor infertility and severe oligozoospermia.

Author

Tu, Chaofeng, Meng, Lanlan, Nie, Hongchuan, Yuan, Shimin, Wang, Weili, Du, Juan, Lu, Guangxiu, Lin, Ge, and Tan, Yue-Qiu

Subjects

*MISSENSE mutation, *MALE infertility, *OLIGOSPERMIA, *HUMAN genes, *PROTEINS, *RESEARCH, *GENETIC mutation, *RESEARCH methodology, *GENETIC testing, *CASE-control method, *EVALUATION research, *MEDICAL cooperation, *INFERTILITY, *COMPARATIVE studies, *GENOTYPES, *GENES, *GENETIC techniques, *CONSANGUINITY, *GENEALOGY, *DISEASE complications

Abstract

Objective: To identify the genetic cause of male factor infertility characterized by severe oligozoospermia.Design: Genetic studies.Setting: Medical university.Patient(s): Two infertile brothers with severe oligozoospermia in a consanguineous Han Chinese family, 414 additional patients with oligo-/azoospermia, and 223 fertile (control) subjects.Invention(s): None.Main Outcome Measure(s): Genetic analyses using whole-exome and Sanger sequencing were performed for two brothers with severe oligozoospermia. The effects of an identified candidate causative mutation were investigated in silico and in vitro. Whole-exome sequencing screening for the candidate mutation was conducted in 414 patients with oligo-/azoospermia and 223 fertile subjects.Result(s): A homozygous missense variant (NM_080746:c.A257C: p.H86P) in RPL10L was identified in the two affected brothers and shown to cosegregate with the severe oligozoospermia phenotype. The mutation was absent in public databases, including the 1000 Genomes Project and the Exome Aggregation Consortium. All queried databases predicted the mutation to be damaging, consistent with the fact that it decreased protein levels in vitro. Subsequent mutation screening identified three additional heterozygous RPL10L mutations in three of 414 subjects with oligo-/azoospermia, but no RPL10L mutations among 223 fertile subjects.Conclusion(s): Our findings implicate RPL10L as a novel candidate gene in the pathogenesis of human male factor infertility and severe oligozoospermia. [ABSTRACT FROM AUTHOR]

Published

2020