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Application of third-generation sequencing technology for identifying rare α- and β-globin gene variants in a Southeast Chinese region
BMC Medical Genomics volume 17, Article number: 241 (2024)
Abstract
Background
Third-generation sequencing (TGS) based on long-read technology has been gradually used in identifying thalassemia and hemoglobin (Hb) variants. The aim of the present study was to explore genotype varieties of thalassemia and Hb variants in Quanzhou region of Southeast China by TGS.
Methods
Included in this study were 6,174 subjects with thalassemia traits from Quanzhou region of Southeast China. All of them underwent common thalassemia gene testing using the DNA reverse dot-blot hybridization technology. Subjects who were suspected as rare thalassemia carriers were further subjected to TGS to identify rare or novel α- and β-globin gene variants, and the results were verified by Sanger sequencing and/or gap PCR.
Results
Of the 6,174 included subjects, 2,390 (38.71%) were identified as α- and β-globin gene mutation carriers, including 40 carrying rare or novel α- and β-thalassemia mutations. The αCD30(−GAG)α and Hb Lepore-Boston-Washington were first reported in Fujian province Southeast China. Moreover, the βCD15(TGG> TAG), βIVS−II−761, β0-Filipino(~ 45 kb deletion), and Hb Lepore-Quanzhou were first identified in the Chinese population. In addition, 35 cases of Hb variants were detected, the rare Hb variants of Hb Jilin and Hb Beijing were first reported in Fujian province of China. Among them, one case with compound αααanti3.7 and Hb G-Honolulu variants was identified in this study.
Conclusion
Our findings may provide valuable data for enriching the spectrum of thalassemia and highlight the clinical application value of TGS-based α- and β-globin genetic testing.
Introduction
Thalassaemia is a worldwide hereditary blood disorder affecting globin chain synthesis, which results in the unbalanced globin chain production, leading to ineffective erythropoiesis, increased hemolysis, and deranged iron homoeostasis [1, 2]. The α- and β- thalassemia are the most common thalassemia, showing high prevalences in the regions such as Mediterranean, Middle East, Indian subcontinent, Southeast Asia and South China [3, 4]. The incidence of thalassemia in Fujian province of Southeast China is about 6.8% [5, 6]. Quanzhou, which has the largest population in Fujian, shows a notable diversity and complexity of thalassemia and hemoglobin (Hb) variants. Rare and novel α- and β-globin gene variants have been increasingly identified in Quanzhou region [7,8,9,10] .
No effective medical treatment for thalassemia intermedia or major is available at present. Conventional thalassemia gene detection before marriage or pregnancy or prenatal diagnosis is the most effective and low-cost intervention mean to prevent and control of the birth defect of thalassemia major or intermedia. However, conventional thalassemia genetic detection based on DNA reverse dot blot hybridization and gap-PCR often leads to misdiagnosis of rare and novel thalassemia [11]. In recent years, the third-generation sequencing (TGS) based on long reads has been used in identifying α- and β-globin gene variants, manifesting remarkable advantages in identifying single-nucleotide variants, indels and structural variants [12, 13]. A prospective study conducted by Xu et al. [14] has demonstrated the application value of TGS technology in molecular diagnosis of thalassemia. Subsequently, a series of studies has reported more rare or novel thalassemia by using TGS [15,16,17] .
The aim of the present study was intended to identify rare α- and β-globin gene variants in Quanzhou of Southeast China by using the TGS technology, hoping that our experience and practice could help establish a more optimized method for the prevention and treatment of thalassemia.
Materials and methods
Samples
This prospective study enrolled 6,174 subjects with positive hematological screening results or one of the couples was identified as a thalassemia carrier from April 2021 to October 2023 at Quanzhou Women’s and Children’s Hospital, excluding those reported in our previous case reports from January 2013 to March 2021 [8]. They included 2,595 males and 3,579 females ranging in age from newborns to 54 years. All cases deny recent blood transfusions within 14 days, and no genetic relationship was exists in all samples. No included subject received transfusion within 14 days before testing, and no genetic relation existed between the samples. Informed consent was obtained from all subjects before conventional thalassemia gene detection. Subjects who were suspected as a rare thalassemia or Hb variants carriers (individuals with positive hematological screening results but elicited negative conventional thalassemia gene testing results) were subjected to α- and β-globin gene sequencing based on TGS technology. This study was approved by the ethics committee of The Women’s and Children’s Hospital of Quanzhou (No.2021No.61).
Hematological screening analysis
Routine blood analysis and Hb electrophoresis were carried out for hematological screening analysis. Approximately 4 ml peripheral blood was collected from each subject and anticoagulated with EDTA-K2. Routine blood detection was conducted using an automated cell counter (Sysmex XS-1000i; Sysmex Co., Ltd., Kobe, Japan). The Hb components were analysed by Hb electrophoresis (Sebia, Evry Cedex, France). Positive hematological screening results that met one of the following indexes were diagnosed (which was only suitable for individuals older than 2 years) [8]: a mean corpuscular volume (MCV) ≤ 82 fl., and/or a mean corpuscular hemoglobin (MCH) ≤ 27 pg, and/or Hb A2 levels ≥ 3.4% or ≤ 2.6%, or an Hb F value ≥ 2.0%. All patients with positive hematological analysis results underwent thalassemia gene testing.
Conventional thalassemia gene testing
About 2 ml peripheral blood was collected from each of the enrolled subjects for conventional thalassemia gene testing. Genomic DNA was extracted using the automatic nucleic acid extractor (Ruibao Biological Co., Ltd., Taiwan). Twenty-three common genotypes of α- and β-thalassemia mutations were identified in the Chinese population using the PCR reverse dot-blot hybridization technique (PCR-RDB) [18], including the deletional (-α3.7, -α4.2, --SEA) and non-deletional α-thalassaemia mutations (αCSα, αQSα and αWestmeadα), and 17 common β-thalassemia mutations: CD41-42(-TCTT), IVS-II-654(C > T), − 28(A > G), CD71/72(+ A), CD17(AAG > TAG), CD26(GAG > AAG), CD43(GAG > TAG), − 29(A > G), CD31(-C), − 32(C > A), IVS-I-1(G > T), CD27/28(+ C), − 30(T > C), CD14-15(+ G), Cap + 40–43(–AAAC), initiation codon(ATG > AGG) and IVS-I-5(G > C) [7].
TGS and data analysis
The peripheral blood samples from 127 subjects who were suspected as rare globin gene variant carriers were sent to Berry Genomics laboratory for TGS, which was performed based on the PacBio Sequel II platform for α- and β-globin gene detection as described in our previous report [16]. In brief, the purified DNA samples were quantified using the Qubit dsDNA BR assay kit (ThermoFisher Scientific). Then, optimized primers were used to generate specific amplicons that encapsulate known structural variation regions, and single nucleotide variation in the α- and β-globin gene. Double barcode adapters were ligated to the 5’ and 3’ ends after purification and end repair, and then Sequel Binding and Internal Ctrl Kit 3.0 (PacBio) was used to prepare SMRT bell libraries. Finally, third-generation sequencing was performed on the PacBio Sequel II System after loading primed DNA-polymerase complexes onto the SMRT cells [16].
By referring to alignment of the subreads, the consensus circular sequence was mapped to the GRCh38 reference and variants called (FreeBayes software, version 1.2.0). WhatsHap (version 0.18) software was used for Linkage analysis (in cis or trans) in the long read based phasing. Alignments of variant and wild-type molecules was manifested by Integrative Genomics Viewer [16].
Sanger sequencing
Sanger sequencing was performed to verify the globin gene variants detected by TGS. Specific primers according to the known DNA sequences were designed to perform PCR. All the designed primers were synthesized by Invitrogen (Shanghai) Trade Co., Ltd. The operation process of Sanger sequencing was performed following our previous study [16].
Results
The detection rate of α- and β-thalassaemia
In our study, 2,390 subjects carrying α- and β-thalassemia mutations were identified, including 1,615 cases with α-thalassemia variants, 719 cases harboring β-thalassaemia variants, and 56 cases with both α- and β-thalassaemia, reaching a total detection rate of 38.71% (2,390/6,174), and the α-thalassemia, β-thalassaemia and complex α- and β-thalassaemia detection rate were 26.16%, 11.65% and 0.91%, respectively. Among these, 2,349 subjects with common α- and β-thalassemia mutations were identified by conventional thalassemia gene testing, reaching a positive thalassemia detection rate of 38.05% (2,349/6,174). In addition, 40 cases with rare or novel thalassemia mutations were identified by TGS, and a case with --SEA/αα that missed the diagnosis by conventional PCR-RDB technology but later was identified by TGS.
Common and rare α-thalassemia variants
As delineated in Table 1, in the 1,615 subjects diagnosed with α-thalassemia, the --SEA/αα (70.84%) genotype was the most prevalent deletional mutation, followed by -α3.7/αα (18.64%) and -α4.2/αα (3.65%). The most common non-deletional mutation was αQSα/αα (1.55%), followed by αCSα/αα, and αWestmeadα/αα, with frequencies 1.30% and 0.43%, respectively. Besides, 29 cases that may cause Hb H disease were detected, among which, -α3.7/--SEA was the most common (1.18%). A patient with homozygous αCS was also classified as having Hb H disease, who was a female and exhibited a remarkably low level of Hb (86 g/L), slightly low level of MCV (81fL) and MCH (25.2pg), and a slightly increased level of serum iron (28.36 µmol/L).
In this study, including 10 genotypes of rare α-globin gene variants, were diagnosed by TGS. Notably, --THAI/αα manifested a higher frequency. In addition, αCD30(−GAG)α was first reported in Fujian province South China. To the best of our knowledge, the complex genotype of αIVS−II−119(−G)(+CTCGGCCC), IVS−II−55(T> G)α/--SEA and a case compound αααanti3.7 with Hb G-Honolulu were first identified in the Chinese population (Figs. 1 and 2). In addition, the rare variants of --FIL/αα, ααCD15/αα, and ααCD117/118/αα were identified again in Quanzhou region of Southeast China.
Common and rare β-thalassemia variants
A total of 719 cases were diagnosed as β-thalassemia, among which βIVS−II−654/βN (36.02%) and βCD41–42/βN (26.01%) were the most common β-thalassemia mutations, followed by βCD17/βN (19.61%), βCD26/βN (5.70%), and β−28/βN (3.48%), which accounted for about 90.82% of β-thalassemia variants (Table 2). In this study, we also identified 7 cases of β-thalassemia intermedia or major, with βIVS−II−654/βIVS−II−654 being the most common genotype.
In addition, 24 cases including 12 genotypes of rare β-thalassemia variants were identified, of which SEA-HPFH was the most frequent (Table 2). Among them, the rare βCD54–58/βN and βCD53/βN were diagnosed again in Quanzhou region using TGS, while, the Chinese Gγ+(Aγδβ)0 had not been described in Quanzhou region before (Figs. 3 and 4). The Hb Lepore-Boston-Washington identified in this study was the first reported case in Fujian province of Southeast China. Moreover, the βCD15(TGG> TAG), βIVS−II−761, β0-Filipino(~ 45 kb deletion), and Hb Lepore-Quanzhou were first reported in the Chinese population by us.
Compound α- and β-thalassemia variants
Of the 6,174 enrolled subjects, 56 cases (0.91%) were diagnosed as compound α- and β-thalassemia, among which --SEA/αα/βIVS−II−654/βN, -α3.7/αα/βCD41–42/βN and -α3.7/αα/βCD17/βN were the three most prevalent genotypes (Table 3).
Hb variant genotypes
TGS was also carried out to confirm the exact hemoglobin variants in subjects with abnormal Hb band(s). Thirty-five cases of Hb variants were detected, including 11 cases of Hb Q-Thailand [CD74(GAC > CAC)], 2 cases of Hb G-Honolulu [CD30(GAG > CAG)], one case of Hb Beijing [CD16(AAG > AAT), and one case of Hb Jilin [CD139(AAA > CAA)], all of which were induced by α-globin gene mutation. In addition, 17 cases of Hb New York [CD113(GTG > GAG)], and three cases of Hb J-Bangkok [CD56(GGC > GAC)] that caused by β-globin gene mutation were identified.
Discussion
Of the 6,174 subjects with suspected thalassemia traits, 1,615 (26.16%) were identified as harboring α-thalassemia variants, 719 (11.16%) as harboring β-thalassemia variants, and 56 (0.91%) as harboring both α- and β-thalassemia, with an overall detection rate of 38.71% (2,390/6,174)]. Notably, α-thalassemia manifests a higher incidence than β-thalassemia, and --SEA/αα, -α3.7/αα and -α4.2/αα were the most common α-thalassemia genotypes, which is consistent with the neighboring provinces of China, and also consistent with the other previous studies in Quanzhou region [8, 18,19,20,21].
In this study, we identified 1,615 subjects with α-thalassemia mutations, among them, the most common non-deletional mutation was αQSα/αα, followed by αCSα/αα, and αWestmeadα/αα. However, αCS was reported to be the most prevalent non-deletional α-thalassemia in Southeast Asia, and αWestmead was displayed a more higher incidence in Guangxi province of China [20]. Patients with compounded heterozygous or homozygous of αQS and αCS are likely to develop moderate anemia similar to Hb H disease [22]. Our present study identified a case of homozygous αCS exhibiting remarkable moderate anemia similar to Hb H disease, which is consistent with a previous study [22]. As such, couples both carrying αCS should be recommended for performing prenatal thalassemia gene testing after pregnant. Of the 16 cases identified by TGS, 10 belong to the rare α-thalassemia genotype. The --THAI/αα manifested a higher frequency in the rare α-thalassemia genotype, which is also consistent with the previous studies [7, 8] suggesting that TGS could be recommended as a routine method for detection of --THAI in Quanzhou region. The αCD30(−GAG) is a rare HBA2 globin gene variant with few reports available, which could be used as a predictor of α+ or α0-thalassemia according to IthaGenes database. Previous studies reported that patients with αCD30(−GAG) combined with deletional α0-thalassemia were likely to develop mild to severe anemia [23, 24]. In the present study, we described the αCD30(−GAG) again in the Chinese population, and for the first time in a cohort in Fujian province. In addition, our finding first displayed a complex genotype of αIVS−II−119(−G)(+CTCGGCCC), IVS−II−55(T> G)α/--SEA in a Chinese pediatric patient with normal hemoglobin value (114 g/L) and a slightly low level of mean corpuscular hemoglobin (MCH, 26.8pg). In addition, we identified a patient with IVS-II-119(-G)(+ CTCGGCCC) and IVS-II-55(T > G) in HBA2 located in cis by TGS, who exhibited normal hematological screening results, suggesting that both variants in α2 may be benign variants. Moreover, a rare case of compound αααanti3.7 with Hb G-Honolulu was first identified in Chinese population with normal hematological screening results.
In the present study, we identified 719 cases carrying β-thalassemia variants, and the most frequent mutation was IVS-II-654(C > T) and CD41-42(-TCTT), which is similar with the finding in other regions of South China [5, 19, 21]. However, in Yunnan province, CD26(G > A) was reported to be the most frequency β-thalassemia mutation [25]. In the present study, we also identified 7 cases with β-thalassemia intermedia or major were also identified, with a detection rate of 0.11%(7/6,174), indicating that a more optimized and comprehensive thalassemia prevention and control method should be carried out. Moreover, we also identified 12 genotypes of rare β-thalassemia variants, including βCD15(TGG> TAG) which is known as rare variant condition that may lead to β0-thalassemia and has been frequently reported in Iran, Pakistan and India [26,27,28]. Interestingly, it is for the first time that we described the rare βCD15(TGG> TAG) variant in the Chinese population, and it is also for the first time that we displayed an extremely rare variant of IVS-II−761 (HBB: c.316–90 A > G) in the Chinese population, knowing that βCD15(TGG> TAG) may lead to β+ or β0-thalassemia, which was first discovered in the United States of America [29]. Interestingly, the patient with IVS-II-761 (HBB: c.316–90 A > G) exhibited low levels of MCV (68fL), MCH (19.7pg), and Hb A2 (1.5%), which may result in β-thalassemia. Furthermore, this study also firstly present a rare deletional Filipino (~ 45 kb deletion) in the Chinese population, which was mentioned in our previous study [30]. This finding may further confirm the mobility and complexity of the population in Quanzhou region. The Filipino (~ 45 kb deletion) was first reported in a Filipino family [31]. A previous study conducted by Tan et al. [32] reported that the Filipino (~ 45 kb deletion) caused 73.3% of β-thalassemia in the Orang Asli in Sabah and Sarawak, which are indigenous/aboriginal peoples in East Malaysia. It was found in our study that the variants of IVS-II−806 (HBB: c.316−45G > C) and IVS-II−672 (HBB: c.316–179 A > C) exhibited variable hematological profiles, but they would lead to β-thalassemia or not needs more investigation.
Notably, we identified 11 cases of δβ-thalassemia in this study, among which SEA-HPFH was the most frequently detected mutation, which may lead to δβ-thalassemia. This finding is consistent with our previous study [8]. It was also for the first time that we identified another rare δβ-thalassemia of Chinese Gγ+(Aγδβ)0 in Quanzhou region, although it has been reported in Chinese populations of other regions [33]. Also, we identified a novel 7.414 kb deletion NG_000007.3:g.63511_70924del that partially covers HBB and HBD globin genes and may cause δβ-thalassemia in Quanzhou region, and we named it as Hb Lepore-Quanzhou [34]. In addition, we first described four cases of Hb Lepore variant (NG_000007.3:g.63633_71046 del) with one bp different with Hb Lepore-Boston-Washington, which has been reported by our previous study [35]. More attention should be paid to the screening and diagnosis of the rare δβ-thalassemia, knowing that homozygous δβ-thalassemia or co-occurring heterozygosity with β-thalassemia may lead to β-thalassemia intermedia or major.
In this study, we identified 35 cases of Hb variants, including Hb New York and Hb Q-Thailand as the most common two hemoglobin variants. Notably, both the rare Hb Jilin [α139(HC1)Lys > Gln (AAA > CAA); HBA2:c.418 A > C] and Hb Beijing [α16(A14)Lys > Asn (AAG > AAT); HBA2:c.51G > T] detected in the present study were first reported in Fujian province, though they were mentioned in our previous study [36]. The Hb Jilin is an extremely rare α-chain variant, which was only occasionally reported in the literature [37]. In addition, Hb Beijing is also a rare condition, with few reports available in the literature [38, 39].
By using the TGS technique, we identified a diverse range of α- and β-globin gene variants in the present study, among which --SEA/αα was diagnosed as a common genotype by TGS, which was missed in the conventional thalassemia gene testing. This study further has strengthened the application value of TGS, suggesting that TGS may prove to be a powerful tool for the diagnosis of common and rare α- and β-globin gene variants.
In this study, we succeeded in identifying rare α- and β-globin gene variants by TGS in Quanzhou region of Southeast China, including a variety of thalassemia and Hb variants such as βCD15(TGG> TAG), βIVS−II−761, β0-Filipino (~ 45 kb deletion), Hb Lepore-Quanzhou, Hb Jilin and Hb Beijing. These findings expanded the prevalence and spectrum of thalassemia in Fujian province of Southeast China, suggesting that the detection of thalassemia genes based on TGS could be used as a first-line tool for globin gene variant detection.
Data availability
The datasets used and/or analyzed during the current study are available from the corresponding author by reasonable request.
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Acknowledgements
We wish to express our appreciation to Quanzhou Science and Technology, Fujian Provincial Key Laboratory of Prenatal Diagnosis and Birth Defects and Huaqiao University Joint of Hospital and University projects for funding this work. We also express our appreciation to the patients who participated in this study.
Funding
This research was supported by Quanzhou City Science and Technology Project (no.2020N049s); Huaqiao University Joint of Hospital and University Innovation Project (no.2021YX005) and Fujian Provincial Key Laboratory of Prenatal Diagnosis and Birth Defects open project (no.cqzdsys-2022-01).
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JZ and JW wrote the article; NH performed participants recruitment and analyzed the data; YZ performed specific gap-PCR amplification and DNA sequencing; JW, LX and JZ revised and polished the paper. All authors have approved the final article.
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This study was approved by the ethics committee of the Quanzhou Women’s and Children’s Hospital (2021No.61). We ensured that all patients participating in this study signed written informed consent for publication of their genetic data and other relevant information.
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All patients signed written informed consent to participate in this study and agreed for their relevant data and information to be used for scientific research.
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Zhuang, J., Wang, J., Huang, N. et al. Application of third-generation sequencing technology for identifying rare α- and β-globin gene variants in a Southeast Chinese region. BMC Med Genomics 17, 241 (2024). https://doi.org/10.1186/s12920-024-02014-2
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DOI: https://doi.org/10.1186/s12920-024-02014-2