| Literature DB >> 23961874 |
Maria Kahn, Nicole LaRue, Pooja Bansil, Michael Kalnoky, Sarah McGray, Gonzalo J Domingo.
Abstract
BACKGROUND: Glucose-6-phosphate dehydrogenase (G6PD) deficiency is a common human enzyme deficiency. It is characterized by abnormally low levels of G6PD activity. Individuals with G6PD deficiency are at risk of undergoing acute haemolysis when exposed to 8‒aminoquinoline-based drugs, such as primaquine. For this reason it is imperative to identify individuals with G6PD deficiency prior to administering these anti-malarial drugs. There is a need for the development and evaluation of point-of-care G6PD deficiency screening tests suitable for areas of the developing world where malarial treatments are frequently administered. The development and evaluation of new G6PD tests will be greatly assisted with the availability of specimen repositories.Entities:
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Year: 2013 PMID: 23961874 PMCID: PMC3765399 DOI: 10.1186/1475-2875-12-286
Source DB: PubMed Journal: Malar J ISSN: 1475-2875 Impact factor: 2.979
Characteristics of the 31 specimens used to evaluate G6PD activity within cryopreserved red blood cells [[16]]
| 6 | 4 | 10 | 6 | 3 | 9 | ||
| 0 | 3 | 3 | - | 4 | 4 | ||
| 15 | 3 | 18 | 15 | 3 | 18 | ||
| 21 | 10 | 31 | 21 | 10 | 31 |
G6PD activity was determined by spectrophotometry with a quantitative assay. G6PD activity within red blood cells was observed by flow cytometry.
Mean and standard deviation (SD) of G6PD enzyme activity (in U/gHb) at Day 0 and at thaw date
| | ||||
|---|---|---|---|---|
| 21 (14) | 20 (20) | 10 (10) | ||
| 4.57 (4.22) | 4.40 (3.80) | 4.74 (4.05) | ||
| 4.04 (4.33) | 4.55 (4.68) | 3.91 (3.93) | ||
| 0.53 (0.46) | −0.15 (0.31) | 0.84 (0.09) | ||
| <0.001 | 0.629 | <0.001 | ||
Meana (SD) G6PD activity at Day 0 is the mean of the activities in fresh blood from which cryopreserved aliquots were used over a given time interval. Meanb (SD) G6PD activity at thaw date is the mean of the activities in the cryopreserved specimens thawed over a given time interval.
*Paired t test P value.
Figure 1Correlation in G6PD activity values between fresh specimens (Day 0) and cryopreserved specimens. (A) Direct comparison of G6PD activities for fresh and cryopreserved specimens is shown. The solid line indicates the linear regression fit. (B) Bland-Altman plot for differences in G6PD activity between fresh and cryopreserved specimens.
Figure 2Longitudinal G6PD activity recovered from three cryopreserved aliquots of the same specimen. Data are shown for four specimens, three with normal G6PD activity and one with deficient G6PD activity. Specimens were cryopreserved at a single date in multiple aliquots. Aliquots of cryopreserved specimens were than thawed at multiple dates and analysed for G6PD activity. (A) Absolute G6PD activity at thaw dates after cryopreservation and (B) Difference in G6PD activity from that at Day 0. For easy comparison the dates were normalized to Days 1, 2, and 3 in Figure 2B.
Parameter estimates and robust standard errors for the generalized estimating equations model of quantitative trinity results
| Intercept | −0.50 | 0.350 | 0.153 |
| Time (days) | −0.003 | 0.002 | 0.138 |
| Day 0 Trinity result | 1.04 | 0.040 | 0.000 |
Figure 3Distribution of G6PD activity within red blood cell popoulations of fresh and cryopreserved specimens. Intracellular G6PD activity distributions as indicated by flourscence are shown for (A) a normal male, (B) heterozygous female, and (C) deficient male specimens. Intracellular G6PD activity profiles are shown for Day 0 prior to cryopreservation and two separate dates at which the same specimen was thawed after cryopreservation.
G6PD status after cryopreservation as determined by two qualitative tests compared to status pre-cryopreservation
| | | ||||
| 8 | 0 | 8 | |||
| | 0 | 13 | 13 | ||
| | 8 | 13 | 21 | ||
| | |||||
| 7 | 1 | 0 | 8 | ||
| | 0 | 0 | 5* | 5 | |
| | 0 | 0 | 8 | 8 | |
| 7 | 1 | 13 | 21 | ||
* The five specimens initially characterized as intermediate by the fluorescent spot test were G6PD deficient by the quantitative test.