| Literature DB >> 24788417 |
Mathilde Di Filippo1, Christophe Marçais2, Sybil Charrière3, Oriane Marmontel4, Martine Broyer4, Mireille Delay5, Micheline Merlin5, Axel Nollace4, René Valéro6, Michel Lagarde7, Valérie Pruneta-Deloche7, Philippe Moulin3, Agnès Sassolas1.
Abstract
BACKGROUND: Determination of lipoprotein lipase (LPL) activity is important for hyperchylomicronemia diagnosis, but remains both unreliable and cumbersome with current methods. Consequently by using human VLDL as substrate we developed a new LPL assay which does not require sonication, radioactive or fluorescent particles.Entities:
Mesh:
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Year: 2014 PMID: 24788417 PMCID: PMC4008628 DOI: 10.1371/journal.pone.0096482
Source DB: PubMed Journal: PLoS One ISSN: 1932-6203 Impact factor: 3.240
Subjects features.
| lane | n | Age year | Sex %of men | BMI kg/m2 | Smoker % of smoker | Diabetes % | |
| 0 | Controls | 20 | 51.7 (22–76) | 55 | NA | NA | 0 |
| 1 | HTG without mutation group: no mutation in | 15 | 45.3 (13–61) | 73 | 27.1 (21.9–34.7) | 20 | 45 |
| 2 | HTG minor polymorphism group: | 20 | 48.4 (23–80) | 80 | 27.6 (17.8–34.0) | 42 | 50 |
| 3 | HTG mild mutation group: homozygous mutation of | 7 | 42.3 (36–50) | 71 | 26.0 (20.3–32.0) | 60 | 14 |
| 4 | HTG mild mutation group and polymorphism: heterozygous mutation of | 8 | 48.4 (32–64) | 50 | 27.5 (21.7–40.0) | 33 | 38 |
| 5 | HTG major mutation group: homozygous mutation of | 5 | 23.3 (5–41) | 60 | 20.1 (19.1–21.0) | 33 | 33 |
| 6 | Patients with anti-LPL antibodies and low LPL activity | 3 | 54.0 (35–70) | 67 | 22.1 (21.8–22.3) | NA | NA |
n effective of the group.
NA not available.
Mean (range) or %.
Figure 1Kinetics and linearity.
Figure 1A. PHLA and HL kinetics in 3 patients. LPL+HL (line); HL (dotted line); Patient 1 (triangle); Patient 2 (circle); Patient 3 (square); Patient 4 (vertical line). Figure 1B. Linearity test. Patient 1(black diamond); Patient 2 (white square); Patient 3 (grey triangle); Patient 4 (black square); Patient 5 (grey square); Patient 6 (grey circle).
Figure 2Correlation between LPL activity assays in TVHTG and controls patients.
Figure 2A. Correlation with conventional method (n = 26, r = 0.88, p<0.001). y = 8.93× + 1.21; R2 = 0.77. Figure 2B. Distribution of LPL activity in TVHTG patients and controls subjects. TVHTG patients (grey square); controls (black square).
Figure 3LPL activity and molecular diagnosis.
$ 3 diabetic compound heterozygous patients ([p.Q139X];[p.S19W polymorphism]); * patient with anti-LPL antibodies and heterozygous mutation of LPL gene; £ Triglyceridemia determined the day of LPL activity measurement.