Repeat Whole Blood Donation Correlates Significantly with Reductions in BMI and Lipid Profiles and Increased Gamma Glutamic Transferase (GGT) Activity among Nigerian Blood Donors ()
1. Introduction
The health benefits of screening for fatty liver and other components of the metabolic syndrome seems as necessary as performing tests for viral hepatitis B and C infections on the blood donors [1]. This is because an estimated 1% - 9% of people who have no symptoms are known to have high liver enzyme levels attributable to non alcoholic fatty liver disease whose risk factors have been known to be obesity, diabetes (insulin resistance), hyperlipidaemia and hypertension [2].
Blood donors are as a whole a protected group against coronary heart disease but according to Bharadwaj [3]there seems to be a reduction in benefit of blood donation as the duration from the date of last donation increases. Frequent blood donations have been reported to reduce the risk of myocardial infarction [4] and this is attributed to the reduction in the iron load with each blood donation [5]. Apart from iron, other biochemical parameters like gamma glutamic transferase (GGT) and lipid parameters play prominent roles in heart disease.
GGT is present in hepatocytes and biliary epithelial cells. The normal range is 0 - 50 U/L in men and 0 - 35 U/L in women. GGT elevation is the most sensitive marker of hepatobiliary disease. However, its routine clinic use is not recommended as it cannot by itself indicate a specific cause of liver disease. Elevated GGT in conjunction with alkaline phosphatase usually points to hepatobilliary injury [5-7]. Serum GGT activity has commonly been interpreted as a marker of alcohol consumption or liver disease [8].
A blood donor who indulges in unhealthy lifestyle of alcohol consumption may develop liver problem unnoticed, thereby constituting a risk in the blood donor pool. On the other hand, GGT is central to the extracellular catabolism of glutathione (GSH), a low molecular weight sulfhydryl compound which is a scavenger of oxygen free radicals and plays a key role in protecting against both intracellular and extracellular oxidative stress [9, 10]. However, GGT has been widely reported to be high in chronic heart failure patients and is also associated with disease severity [11].
Most studies are centered on the effect of blood donation on iron parameters probably due to the adverse consequences of anaemia or iron deficiency anemia [12,13]. Considering the lifestyle of most of our blood donors vis-a-vis excessive alcohol intake, smoking, etc. which has direct effect on hepatocytes, It therefore become necessary to look beyond anaemia to ensure a safety donor pool with minimal consequences on the blood recipients. This study was therefore aimed at determining the gamma glutamic transferase activity and lipid profiles of repeat donors in our setting for the purpose of establishing the baseline values.
2. Materials and Methods
2.1. Subjects
Two group of subjects participated in this study. The first group consisted of repeat donors (those who have donated blood at 3 to 4 times in a year for at least two consecutive years). The second group was the first time donors and consisted of men who were registered as new blood donors without any prior donations. Informed consent was received from each of the 103 repeat donors as well as from the 90 first time donors. The weights and heights of the participants were obtained and the body mass index (BMI) calculated as weight/height2. The blood pressure of the participants was also taken from each of them.
Four (4) milliliters of venous blood sample was collected from each subject, transferred into a plain bottle and used for biochemical analysis. Clotted blood samples in plain bottles were centrifuged at 2500 g for 5 minutes to separate the serum used for the analysis.
2.2. Gamma-Glutamyltransferase (GGT) Determination
GGT concentration was determined using human commercial kit which is based on the ability of the GGT in the sample to catalyze the transfer of the glutamyl group from GLUP-C to glycylglycine. The amount of 5-amino- 2-nitrobenzoate formed is proportional to GGT activeity and measured kinetically at 405 nm.
1.0 ml of the reagent containing glycylglycine, GLUPA-C, sodium azide and tris-buffer was put into test and control tubes already incubated at 37˚C. This was followed by the addition of 100 µl of the serum sample into the tubes. The contents of the tubes were mixed and incubated for 1 minute. The absorbance of the test and control were measured against the distilled water blank at 405 nm. The absorbance was repeated after 1 minute and the mean difference per minute multiplied by 1158 to obtain the result in microlitre (µl).
2.3. Lactate Dehydrogenase (LDH) Determination
LDH determination using the human kit is based on catalyses of the oxidation of lactate to pyruvate with simultaneous reduction of nicotinamide adenine dinucleotide (NAD) to NADH. The rate of NAD reduction can be measured as an increase in absorbance at 340 nm. This rate is directly proportional to LDH activity in serum.
1.0 ml of the reagent containing a mixture of NAD, L-lactate and buffer was put into test and control tubes already incubated at 37˚C. 50 µl of serum sample was added to these tubes, mixed and incubated for 30 seconds. The absorbance (A1) reading was done, then the tubes were re-incubated for another 1 minute and the absorbance (A2) measured. The change in the absorbance (A2-A1) was multiplied by the factor 3376 to obtain the result in microlitre. The absorbances of the test and control were measured against the distilled water blank at 340 nm.
2.4. Triglycerides Determination
10 µl each of sample and standard solutions were added to 1000 µl of the reagent containing lipases and quinoneimine indicator. It was mixed and incubated for 5 minutes at 37˚C. The absorbance of the sample and standard were measured against the reagent blank within 60 minutes.
2.5. Total Cholesterol Determination
1000 µl of the reagent containing a mixture of esterase, peroxidase and quinoneimine indicator was added to 10 µl of distilled water, standard and serum sample respectively in three different test tubes. The contents were mixed and incubated for 5 minutes at 37˚C. The absorbance of the sample and of the standard against the blank at 500 nm was determined.
2.6. High Density Lipoprotein (HDL) Cholesterol
1000 µl of the reagent was added to 100 µl of distilled water, supernatant from sample and standard supernatant respectively in three different test tubes. The contents were mixed and incubated for 5 minutes at 37˚C. The absorbances of the sample and of the standard were measured against the reagent blank at 500 nm. Low density lipoprotein (LDL) Cholesterol was calculated as follows:
LDL = Total Cholesterol-Triglycerides/2.2-HDL Cholesterol.
2.7. Statistical Analysis
The statistical analysis was done using SPSS statistical package (version 15 Chicago, IL, USA). All results were calculated as mean ± SD and a P value of ≤ 0.05 was considered statistically significant. Mean values were compared using the paired t-test. Pearson correlation analysis was performed to determine the factors affecting changes in donor parameters after repeated blood donations.
3. Results
A total of two hundred and fourty three (243) blood donors participated in this study. Ninety (37.0%) of them were first time donors while one hundred and fifty three (63.0%) were repeat donors. Majority of them (73.3%) were under 30 years of age while 26.7% were between 31 - 35 years. None of the blood donors was above 35 years. All the donors in the repeat category were under 30 years of age. All the blood donors were males.
Table 1 shows the blood pressure, age, BMI and biochemical parameters of the 243 blood donors who participated in the study. There was no significant difference in the age and blood pressure parameters. The BMI values of 24.4 ± 2.4 kg/m2 in the first time donors was significantly higher than the 21.7 ± 1.7 kg/m2 obtained in repeat donors (P < 0.001). Gamma glutamyl transferase was significantly higher in repeat donors (70.5 ± 13.5 µl) than the first time donors (62.5 ± 13.3 µl) (P < 0.05). Lactate dehydrogenase enzyme showed no significant changes in the values between the two groups (P = 0.948).