Association of vitamin D receptor gene BsmI (A>G) and FokI (C>T) polymorphism in gestational diabetes among Saudi Women

Objective: Vitamin D receptor (VDR) gene polymorphism have a role in diabetes mellitus pathogenesis. Present study was conducted to determine VDR gene variants among Saudi gestational diabetics (GDM) in Madina, KSA. Methods: This cross sectional study was conducted on 112 GDM patients and 218 normal healthy control. Age, body mass index and blood pressure levels were recorded. Serum triglycerides (mg/dl), total cholesterol, HDL-cholesterol, LDL-cholesterol, fasting blood glucose FBG and post-prandial blood glucose PPBG were estimated. Extracted DNA template was amplified by PCR reaction and genotyped for single nucleotide polymorphism of BsmI and FokI by restriction fragment length polymorphism-PCR (RFLP-PCR) analysis. Results: FBG and PPBG levels in GDM patients were significantly elevated by +48.6% and +50%, respectively (P=0.005). Serum triglycerides, total cholesterol and LDL-cholesterol (mg/dl) levels in GDM patients were elevated significantly by +40.5% (P=0.005), +16% (P=0.01) and +30.8% (P=0.005), respectively. Serum HDL-cholesterol (mg/dl) showed significant decline by -10.5%. FokI VDR genotypes showed association with PPBG (P=0.05) among GDM patients. The Ff, FF and ff genotype percentage among GDM patients was 48.2%, 30.4% and 21.4%, respectively. FokI (F and f) and BsmI (B and b) alleles frequency showed no significant difference between GDM patients and control. Percentage BsmI and FokI total homozygous and heterozygous variants among GDM was 45.5% and 81.4%, respectively. Conclusion: VDR BsmI and FokI polymorphic marker not associated with Saudi GDM.


Vitamin D & gestational diabetes
BsmI (A to G), have unknown functional effects. 7ositive association between BsmI (genotype bb) polymorphisms with reduced insulin secretory capacity was reported. 8Diabetics with BB genotype of BsmI allele in VDR gene presented higher levels of C-peptide suggesting association between VDR polymorphism and diabetes. 9estational diabetes (GDM) patients are known to be at greater risk of reduced vitamin D levels as vitamin D was deficient in 70.6% of GDM patients. 10,11This study was carried out in order to investigate association between VDR-BsmI(A>G) and VDR-FokI (C>T) gene polymorphism and risk of GDM among Saudi pregnant women located in Madina-Saudi Arabia.

METHODS
Blood samples were collected from 112 pregnant GDM and 218 normal healthy control Saudi women from outpatient clinic of Ohud hospital, Madina, Saudi Arabia from 11-2013 till 11-2014.Local ethical committee of Medical Applied Sciences faculty, Taibah University, Saudi Arabia approved study protocol and written informed consent was obtained from participants.Age (years), body mass index-BMI (Kg/m 2 ), systolic blood pressure (mm/ Hg) and diastolic blood pressure (mm/Hg) levels were recorded.Serum triglycerides (mg/dl), total cholesterol (mg/dl), HDL-cholesterol (mg/dl) and LDL-cholesterol (mg/dl) levels were estimated using kits from Randox, UK.Fasting blood glucose FBG (mg/dl), post-prandial blood glucose PPBG (mg/dl), were determined using glucose oxidase kit from Randox, UK.Patients screeningwas carried out according to American Diabetes Association guidelines. 12Exclusion criteria included diabetic women, women with multiple pregnancies or diseases as infections, nephropathy, retinopathy,.... etc, and smoking.
Five ml blood sample was collected in EDTA-tube.DNA was extracted using GelElute DNA extraction kit (QIAGEN, Germany) and was checked for purity and concentration. 13DNA samples were all quoted and stored at -20°C till analysis.Restriction fragment length polymorphism (RFLP-PCR) was used to identifyVDR genotypes.Amplified PCR product (10 ml) was digested (37 o C for 20h) with 4U of either BsmI or FokI restriction enzyme (NEB, UK) in 20 µl reaction volume.Digested product was electrophoresed on 2% agarose gel.For statistical analysis, capital letters represented absence and lowercase letters represented presence of BsmI or FokI restriction site; (B/b) and (F/f), respectively.Genotype was determined according to fragments length i.e. homozygote GG(BB) subjects = 650 and 172bp product; heterozygote GA (Bb) subjects = 822, 650and 172bp products and homozygote AA (bb) subjects =822bp product.SNP resulting in A-G substitution in VDR gene intron 8 leads to generation of a BsmI restriction site.Homozygous subjects with alleles containing nucleotide A at this position showed one band at 822 bp and were designated as having bb BsmI genotype.Homozygous subjects with alleles containing G at this position showed 2 bands of 650 and 172bp and were designated as BB.Subjects with heterozygote status showed 3 bands:825, 650 and 172bp and were designated Bb. 14 FokI genotype was determined according to fragments length i.e. homozygote (FF) subjects = 196, 69bp product;heterozygote (Ff) subjects =265, 196 and 69bp products and homozygote (ff) subjects =265bp product.SNP resulting in T-C substitution in exon2 of VDR gene leads to the generation of a FokI restriction site.Homozygous subjects with alleles containing nucleotide T at this position showed an intact 265bp band and were designated as having ff FokI genotype.Homozygous subjects with alleles containing C at this position showed 2 bands of 196 and 69bp (FF Subjects).Heterozygote subjects showed all 3 bands: 265, 196 and 69bp and were designated Ff . 15esults were presented as means±standard error (SE) and number (percentage).Difference between two groups was determined by unpaired Student`s t-test using GraphPad Prism software version 5.0 (USA).Results were considered statistically significant at P ≤0.05.

RESULTS
Total number of 112 GDM patients and 218 healthy pregnant women were recruited in our study.Age, BMI, systolic and diastolic blood pressureshow no statistical significant difference compared to normal control (Table-II).
Fig. 1, shows PCR product of 822 bp for VDR BsmI gene and 265 bp for VDR FokI gene.We compared FokI and BsmI VDR genotypes with demographic and biochemical parameters of GDM patients but we could not achieve significant association of any of the parameters except PPBG (P=0.05) with VDR FokI genotypes (Table-III).
Genotype and allele frequency of VDR FokI and BsmI gene polymorphism in GDM patients and controls showed insignificant differences (Table-IV).Table-V, shows that BsmI total percentage of homozygous and heterozygous variants among GDM patients and control was 45.5% and 81.4%, respectively.FokI total percentage of homozygous and heterozygous variants among GDM patients and control was 78.6% and 84.8%, respectively.

DISCUSSION
Diabetes mellitus has become major health concern worldwide.About 90-95% of the total diabetics are of type 2. 16 Diabetes mellitus affect about 30% of Saudi population.Females <50 years old (gestational age) had greater prevalence than males. 17VDR polymorphism influences susceptibility to type 1 diabetes mellitus, but association with GDM is not yet clear. 18Vitamin D has suggested to be strongly related to pancreatic β-cell function and insulin sensitivity. 8,19It was reported that, no association was noticed between VDR BsmI polymorphism and GDM in Saudi population. 20We analyzed VDR gene BsmI (A>G) and FokI (C>T) polymorphic markers in GDM pregnant Saudi women.It was revealed that, VDR gene polymorphic markers wer enot found to be associated with VDR gene polymorphic markers with type 1 diabetes mellitus. 21enotypes frequencies for wild, heterozygous and homozygous variant of BsmI polymorphic allele among control groups were 0.183, 0.300 and 0.514, respectively, and among GDM patients were 0.545, 0.0980 and 0.357, respectively, with insignificant association (P=0.820).Total homozygous and heterozygous was 0.455 and 0.814 among GDM patients and control, respectively (Table IV & V).It was reported that, BsmI genotype frequencies in GDM Saudi subjects were 0.300, 0.100 and 0.600, respectively; with no significance. 20enotypes frequencies for wild, heterozygous and homozygous variant of FokI polymorphic allele in control were 0.151, 0.298 and 0.551, respectively, and in GDM patients were 0.214, 0.304 and 0.482, respectively, withno significance (P=0.341).Total homozygous and heterozygous was 0.786 and 0.848 among GDM patients and control, respectively (Table IV & V).This is the first time that, VDR gene Fok1 polymorphic allele was analyzed in Saudi GDM subjects.Other studies have revealed that Fok1 genotype frequencies among Indians were 0.437,0.491and 0.07221. 22Both FBG and PPBG did not show significant different between those with wild type and variant allele of both BsmI and FokI gene polymorphism among control and GDM subjects (Table-VI).These findings, are in contrast with results of other studies that showed direct association between BsmI and elevated FBG. 15 An Indian study suggested that, VDR gene polymorphism is associated with type 2 DM. 23e reported no evidence of allelic or genotypic association of the BsmI and FokI of VDR gene with GDM in our studied GDM population.Results obtained by different investigators who studied BsmI polymorphism varied among diabetics.BsmI polymorphism has been linked to susceptibility to diabetes in several countries. 5,24However, studies in other countries could not establish association between BsmI and existence of diabetes. 25,26In type 2 DM, a link between BsmI and the onset of the disease has been found in several countries .27,28but not amongother populations. 29,30These variations may due to ethnic differences in VDR polymorphisms distribution that may have role in diabetes mellitus pathogenesis.

CONCLUSION
Both BsmI (A>G) and FokI (C>T) VDR gene polymorphism showed non-significant association with GDM subjects except for PPBG in case of FokI genotype.Polymorphic marker alleles did not have effect on glycemic of Saudi GDM patients.Further merit investigation will be required to elucidate these findings using larger sample size.
DNA (2 µl) was amplified in 50 µl PCR reaction mixture containing 5 µl10x PCR buffer, 25 mM MgCl 2 , 4 m MdNTPs, 15.M of each primer and 0.5UTaq DNA polymerase.Primers used in this study are listed in Table-I.PCR thermal cycler

Table - I
: Primers used for polymerase chain reaction (PCR)of VDR FokI and BsmI genes.
DR: Vitamin D receptor.

Table -
II: Demographic and biochemical data of GDM patients and controls.

Table III :
Association of various biochemical and clinical parameters with different VDR (BsmI and FokI) genotypes in GDM.Table-IV: Genotypes and allele frequenciesof VDR BsmI and FokI gene polymorphism.