# Analytical validation of a direct lipoprotein(a)-cholesterol assay

**Authors:** Santica M. Marcovina, Spenser Smith, Lizhu Lin, Sotirios Tsimikas

PMC · DOI: 10.1016/j.jlr.2026.101008 · Journal of Lipid Research · 2026-02-23

## TL;DR

This paper describes the development and validation of a new test to measure Lp(a)-C, a type of cholesterol linked to heart disease, which could improve lipid testing in patients with high Lp(a).

## Contribution

The first analytical validation of a direct method to quantify Lp(a)-cholesterol in a certified clinical laboratory.

## Key findings

- The assay showed excellent linearity (R2 = 1.00) and a measuring range of 0.78 to 40.0 mg/dl.
- Lp(a)-C was stable for 3 months at −70 °C and through two freeze-thaw cycles.
- Direct Lp(a)-C correlated strongly with Lp(a) molar concentration (r = 0.93, P < 0.001).

## Abstract

Accurate measurement of lipoprotein(a)-cholesterol [Lp(a)-C] may be useful in interpreting the traditional lipid panel, particularly in patients with high Lp(a). We developed and analytically validated a direct immunocapture ELISA in a Clinical Laboratory Improvement Amendments-certified laboratory for quantifying Lp(a)-C in human plasma using an apolipoprotein(a)-specific monoclonal antibody (LPA4) coupled to magnetic beads. The linearity of the assay was found to be excellent (R2 = 1.00), with % bias ranging from 0.3% (upper limit of quantification) to 16.1% (lower limit of quantification) and coefficient of variation ranging from 3.4% to 16.2%. The analytical measuring range was 0.78 mg/dl to 40.0 mg/dl, and the limit of blank and limit of detection were 0.02 mg/dl and 0.05 mg/dl, respectively. The intra- and interassay coefficients of variation, determined on four quality control samples, ranged from 4.9% to 7.6% and from 12.6% to 15.0%, respectively. No interference was observed from hemolysis (up to 0.71 g/dl), bilirubin (up to 10.1 mg/dl), or triglycerides (up to 1,082 mg/dl. Lp(a)-C was stable for at least 3 months at −70 °C and through two freeze-thaw cycles. Direct Lp(a)-C correlated strongly with Lp(a) molar concentration (r = 0.93, P < 0.001). This study reports the results of the first analytical validation of a direct method to quantify Lp(a)-C, enabling standardized quantification of Lp(a)-C suitable for research studies and clinical trials; additional clinical outcome validation will be required prior to routine clinical implementation.

## Linked entities

- **Chemicals:** bilirubin (PubChem CID 5280352)
- **Species:** Homo sapiens (taxon 9606)

## Full-text entities

- **Genes:** LPA (lipoprotein(a)) [NCBI Gene 4018] {aka AK38, APOA, LP}
- **Diseases:** hemolysis (MESH:D006461)
- **Chemicals:** lipid (MESH:D008055), Lp(a)-C (-), Lp(a) (MESH:D010649), Cholesterol (MESH:D002784), triglycerides (MESH:D014280), bilirubin (MESH:D001663)
- **Species:** Homo sapiens (human, species) [taxon 9606]

## Full text

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## Figures

5 figures with captions in the complete paper: https://tomesphere.com/paper/PMC13022595/full.md

## References

12 references — full list in the complete paper: https://tomesphere.com/paper/PMC13022595/full.md

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Source: https://tomesphere.com/paper/PMC13022595