INTRODUCTION
Glucose-6-phosphate dehydrogenase (G6PD) is an X-chromosome (Xq28)-linked housekeeping cytoplasmic enzyme. It has a redox function as the first enzyme of the pentose-phosphate pathway involving in the generation of NADPH, an electron donor required for many biosynthetic processes or to counter the damaging effects of oxygen radicals [
1,
2]. It is one of the most polymorphic proteins, in which at least 140 mutations have been identified [
3,
4]. G6PD deficiency produces various clinical presentations. It is the most common enzymopathy of humans over 400 million individuals throughout the world, showing as high frequency as 30% in tropical Africa, parts of the Middle East, and Southeast Asia. The G6PD deficient individuals are usually asymptomatic but acute hemolysis may occur with oxidative stress induced by ingestion of drugs, certain type of food, exposing to certain chemical substances or when there is accompanying infection or hypoxia [
5]. Numerous lines of evidence indicate that the geographic correlation of its distribution with the historical endemicity of malaria and suggest that the defect has risen in frequency through natural selection by malaria [
6–
8]. Recently, it was known that studies carried on the Korean population showed no cases representing above severe G6PD deficiency [
9–
11]. The higher frequencies of the defect were reported from Africa, Asia, the Mediterranean region, and the Middle East, owing to recent migrations and perpetual communications. The disorder was also reported from North and South America and even from the European countries [
12].
Although there has been a mixed pattern of repeated increases and decreases, the vivax malaria incidence in Korea has generally shown a plateau (around 1 incidence rate per 100,000) since its re-emerging in 1993 and the highest patient outbreak in 2000 (4,142 confirmed and indigenous cases, 8.98 incidence rate per 100,000) [
13]. Despite such a declined and steady state, there remain tasks to be achieved for vivax malaria elimination from Korea.
In general, it is well established that the spatial extent of vivax malaria overlaps widely with that of G6PD deficiency. The antimalarial licensed for the radical cure and relapse prevention for vivax malaria, is only primaquine. It, unfortunately, can trigger severe hemolytic anemia, particularly in G6PD deficient individuals [
14]. The World Health Organization (WHO) recommends primaquine at a dose of 0.25–0.5 mg/kg of body weight for 14 days in all vivax malaria patients with normal G6PD activity [
15]. G6PD testing is not generally accessible in most malaria-endemic regions. It is, therefore, lower dosages of primaquine are recommended to reduce the risk for the suspected G6PD deficient patients [
16].
As previously documented, due to the low prevalence in Korea, G6PD deficiency testing has not been executed. However, G6PD deficient patients have been continually reported since 1984. G6PD deficiency-related hemolytic anemia patients in Korea Army were confirmed after primaquine administration without G6PD deficiency testing [
11,
17]. In addition, recently, multicultural families have been on the rise due to the increase in immigrants from Southeast Asian countries, where frequency of G6PD deficiency is as high as 30%. In Korea, proportion of the multicultural families is 4.3%, similar to 5% in the countries of the Organization for Economic Cooperation and Development [
18]. Moreover, the multicultural families in Korea mostly composed of maternal immigrants. It is expected that the G6PD deficiency rate of children of these families increase.
This study was aimed to figure out the G6PD deficiency profile of the adolescents in multicultural families and to establish a basis for the G6PD screening test before primaquine administration, and to survey on recognition of the multicultural family center for the G6PD deficients.
MATERIALS AND METHODS
Ethics statement, collection sites and sample collection
This study was reviewed and approved by the Institutional Review Board of the Inha University Hospital (Approval No. 2020-04-004) and conducted according to the principles expressed in the 1964 Helsinki Declaration. This study was conducted with extensive cooperation from the local multicultural family centers and the local public health authorities. In conjunction with the multicultural centers in each province involved in this study, genotype analysis of G6PD, enzyme activity measurement and blood test were performed to investigate G6PD deficiency among the adolescents in multicultural families and the maternal multicultural members from 10 countries. Written informed consents were obtained from participants themselves and their parents or student’s guardians to collect a blood sample prior to personal information talking obtained through interviews and questionnaires. The questionnaire was focused on demographic characteristics analysis and on previous medical history or the composition of the entire family. A total 733 blood samples were collected from the study population: 417 from the adolescents in multicultural families (219 females and 198 males) and 316 from the maternal multicultural members. The blood samples were collected from venous puncture (3 ml in K2EDTA vacutainer tubes), and analyzed using standard quantitative G6PD enzymatic assay.
Determination of G6PD deficiency
G6PD and hemoglobin (Hb) testing by venipuncture was carried out with G6PD quantitative kinetic UV assay using whole blood kit (Cat. No. G6P8905; BEN-Biochemical Enterprise S.r.l., Milano, Italy) according to the manufacturer’s instructions. The blood samples were transferred to the Seoul Clinical Laboratories (Yongin, Korea) within 24 hr after collected under appropriate storage conditions to quantitate enzyme activity of G6PD [
19].
DNA extraction and analysis on G6PD variants
Genomic DNA was extracted from 200 μl of whole blood using QIAamp DNA Blood Mini Kit (Qiagen GmbH, Hilden, Germany) according to the manufacturer’s instruction. Extracted DNA samples were diagnosed using DiaPlexCTM G6PD Genotyping Kit (Asian type, SolGent Co., Ltd., Daejeon, Korea) based on the multiplex allele-specific PCR based assay system for screening G6PD deficiency according to the manufacturer’s instruction. It detects specifically the 7 Asian variants of the G6PD gene via one-step PCR. The variant each produce PCR products of different sizes: Vanua Lava (383 T→C, product size: 154 bp), Mahidol (487 G→A, 337 bp), Mediterranean (563 C→T, 262 bp), Coimbra (592 C→T, 243 bp), Viangchan (871 G→A, 501 bp), Union (1,360 C→T, 803 bp), Canton (1,376 G→T, 681 bp), and Kaiping (1,388G→A, 557 bp). The PCR round was performed under the following conditions: 95°C for 1 min, followed by 35 cycles at 95°C for 30 sec, 60°C for 30 sec, and 72 for 40 sec, and a final extension at 72°C for 5 min. The amplification reaction was carried out in 20 μl volume reactions, including primer volumes (2 μl each of forward and reverse primers, 10 pmole/ml), 12.5 μl of PCR Smart mix, and 3 μl of DNA template. PCR products were resolved by agarose electrophoresis on 1% agarose gel and stained with SYBR Safe DNA GelStainTM (Thermo Fisher Scientific, Waltham, Massachusetts, USA).
DISCUSSION
Vivax malaria is still an important public health problem in Korea, particularly near the DMZ in the northern part of Gyeonggi-do, including Gimpo and Paju, and Gangwon-do [
13]. In fact, vivax malaria elimination in Korea is generally expected to be successful. However, there are a number of points for consideration against malaria elimination. In this globalized era, international intercourses are frequent due to mutual exchanges and travel between many countries. Furthermore, diversification of genetic sources due to each regional genetic characteristic can cause problems in many aspects. There is substantial room for improvement in radical cure policies and practices. Most of the current guidelines for the radical treatment of vivax malaria recommend the use of primaquine (0.25 mg/kg of body weight) for 2 weeks overlapping with the radical treatment with blood schizonticide agents, such as chloroquine (5 mg/kg, 3 times with 12 hr interval after first dose (10 mg/kg) or 5 mg/kg once with 24 hr interval after the first and second doses (10 mg/kg) [
20]. However, the downside of guidelines recommended by the Korea Disease Control and Prevention Agency is that primaquine, which is the only available antimalaria drug that kills dormant liver stages of
P. vivax and prevents its relapse, can be toxic to individuals with G6PD deficiency. Nowadays, no treatment guidelines in Korea have been issued that account for the G6PD deficiency. Several reports presented that no G6PD deficiency was observed using phenotypic- or genotypic-based tests in individuals and young soldiers residing in vivax malaria endemic regions in Korea [
10,
11].
The population of multicultural families consisting of a marriage immigrant or foreigner with Korean citizenship, have been rapidly growing in Korea since 2000. While international migration has become a global phenomenon over recent decades, Korea has experienced this phenomenon relatively recently. Among the registered foreign population in 2018, 6.7% (159,206/2,367,607) were marriage migrants, which were the second largest group, following migrant workers [
21]. 83.2% (132,391/159,206) of the international marriages were between a Korean groom and foreign bride. Consequently, the number of adolescents in multicultural families was 122,212 in 2018 in Korea and tends to continuously increase annually [
22]. Adolescents in multicultural families accounted for 2.2% of the total Korean adolescent population in 2018, which is over 3 times higher than that in 2012 (0.7%) [
22]. In this study, we found overall 7.8% of participants with G6PD deficiency in male adolescent participants. In the case of the marriage immigrant women (the materfamilias population), 3.2% of participants showed G6PD deficiency. The above results suggest that our country should also seriously consider establishing guidelines for prescriptions on primaquine currently in use to treat malaria and to prevent the significant toxic effects accompanying this drug usage.
This study was designed to identify the prevalence of G6PD deficiency in multicultural families in Korea by maternal immigration and strengthen patient care as a strategy for implementing a 5-year action plan to eliminate malaria again. Through this, the government sought to secure evidence for the rapid diagnosis of anemia for the safety of patients. The G6PD deficiency is high in Southeast Asia, the Middle East, the Mediterranean coast, the South Pacific islands and Africa, but the global population migration, inter-country exchanges, and marriage are increasing worldwide. This raises concerns over the development of hemolytic anemia caused by primaquine drugs. In this study, a total of 733 blood samples were collected in 7 counties (Goseong, Yangyang, Haenam, Hampyeong, Hwasun, Boseong, and Yeoncheon) and 2 cities (Donghae and Taebaek) of Korea. On blood samples, a G6PD enzyme activity test using G6PD quantitative kinetic UV assay on whole blood kit was performed. Based on classification by the WHO, 12 severe (<10% of the median enzyme activity) phenotypic participants, 9 moderate (10% to <30%) ones, and 10 mild (30% to <60%) ones were identified and 4.2% of the participants in this study were with G6PD deficiency. Simultaneously with blood collection, hemoglobin levels were measured to monitor whether specimen were anemic. No subject from the regions where were collected in this study had a medical history of vivax malaria infection. The current surveillance has been conducted on malaria non-endemic areas, and it is thought that future investigations into G6PD deficiency in malaria endemic areas, especially the marriage immigrant women (the materfamilias population) and their next adolescent generation including the registered foreign populations, will be needed continuously and with a wide range of targets.
In conclusion, there are at least 6
G6PD variants (Viangchan, Canton, Vanua Lava, Union, Kaiping, unknown mutation (s)) in the population of multicultural families consisting the materfamilias and their adolescents. Possible reasons for the detected other unknown mutated allele variants are that another mutant that were impossible to be identified by the kit used in this experiment can be expected to exist or to be other type mutant. So far, it is acceptable in Korea that G6PD deficiency prevalence is low enough that the risk of antimalaria drug, primaquine-originated G6PD deficiency-mediated hemolytic anemia is relatively negligible. However, in this study, the population of multicultural families, particularly in adolescent population, have carried G6PD deficiency. In addition, although the G6PD deficient individuals with activity <30% of the median value is not identified, large number of military personnel with C1311T/IVS and T93C intron mutations, which are recognized to be associated with G6PD deficiency, were identified [
11]. There are also the recent case reports of G6PD deficiency-mediated hemolytic anemia in the malaria endemic area [
23–
25]. Therefore, when it is considered that the genetic variants in
G6PD associated with enzyme activity deficiency exists in Korean population, that primaquine chemoprophylaxis is carried out routinely in military personnel in the vivax malaria endemic area, and that there are somehow case reports for G6PD deficiency in the endemic area, further regular surveillance of G6PD deficiency and radical treatment guidelines are needed to ensure the safe administration of the unique anti-vivax malaria drug, primaquine.