All that glitters is gold?

Cott, Elizabeth M. Van

doi:10.1002/ajh.21641

Cited by 5 publications

(6 citation statements)

References 12 publications

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“…For wild type (normal) specimens, the error rate of the assays themselves (0.0025% or 1 in 406) appeared to be much lower than the error rate involving accidentally switching the two specimens or typographical errors (some of which may have been errors in in filling out the report form, which is not a form that is used for patients, and laboratories may be less familiar with the format) [49].…”

Section: Laboratory Errorsmentioning

confidence: 91%

“…With bone marrow transplants, if a patient with FV Leiden receives bone marrow from a donor without FV Leiden , DNA tests (using whole blood specimens and thus DNA obtained from white blood cells) will indicate the normal genotype of the donor, but the plasma will continue to show APC resistance, reflecting the true status of the patient. Similar considerations apply if donors carry FV Leiden and the recipient does not [49].…”

Section: Transplant Patientsmentioning

confidence: 98%

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Factor VLeiden

2015

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Factor V Leiden (FV Leiden ) is a common hereditary thrombophilia that causes activated protein C (APC) resistance. This review describes many of the most fascinating features of FV Leiden , including background features, mechanisms of hypercoagulability, the founder mutation concept, the "FV Leiden paradox," synergistic interaction with other thrombotic risk factors, the intertwined relationship between FV Leiden and APC resistance testing, and other, uncommon mutations implicated in causing APC resistance. In addition, there are several conditions where laboratory tests for APC resistance and FV Leiden are or can be discrepant, including lupus anticoagulants, anticoagulants such as direct thrombin inhibitors (dabigatran, argatroban, and bivalirudin) and rivaroxaban, as well as pseudohomozygous, pseudo-wildtype, liver transplant, and bone marrow transplant patients. The laboratory test error rate for FV Leiden is also presented.

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Section: Laboratory Errorsmentioning

confidence: 91%

Section: Transplant Patientsmentioning

confidence: 98%

Factor VLeiden

2015

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“…However, APC‐R assays are cost‐effective, are easily automated, and can detect acquired APC‐R. They also detect pseudohomozygous FVL, detect pseudo–wild‐type FVL, and assess phenotypic FVL thrombophilia in bone marrow or liver transplant patients …”

Section: Recommendations For Testingmentioning

confidence: 99%

“…The FVL polymorphism (R506Q; p.Arg534Gln) is a single‐nucleotide polymorphism (SNP) that is detectable by methodologies designed or adapted for SNP detection, e.g., restriction digestion and allelic discrimination . Various commercially available diagnostic kits exist, although many laboratories still use assays developed in‐house.…”

Section: Genetic Analysesmentioning

confidence: 99%

Recommendations for clinical laboratory testing of activated protein C resistance; communication from the SSC of the ISTH

Moore

Cott

Cutler

et al. 2019

Journal of Thrombosis and Haemostasis

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| INTRODUC TI ONRegulation of fibrin formation through activated protein C (APC) degradation of activated factor V (FVa) and activated FVIII is a major anticoagulant process of hemostasis. In 1993, Dahlbäck et al 1 identified thrombophilic individuals whose plasma showed a poor response to APC in a coagulation assay based on activated partial thromboplastin time (APTT). This was found to be related to an arginine 506 to glutamine substitution in F5 rendering FV resistant to APC inactivation, and called FV Leiden (FVL). 2 Mutations in F5 other than FVL that confer APC resistance (APC-R) with various degrees of clinical severity have been described, although they appear to be very rare. 3 As the original assay was based on APTTs performed on undiluted plasma, it was prone to numerous interferences, so a modification was subsequently proposed that improved sensitivity and specificity by diluting test plasma in FV-deficient plasma, and remains in widespread use. 4-6 Acquired APC-R may occur in the absence of F5 mutations, and represents an independent risk factor for venous thrombosis. 7 APC-R detection has evolved since the original assay and its modification, and this is the first guideline to address clinical laboratory testing recommendations for the wider set of commonly available phenotypic assays. | PRE ANALY TIC ISSUE S | Patient selectionIndiscriminate testing for APC-R is not recommended in unselected patients with venous thromboembolism (VTE). Targeted testing is recommended for those situations in which the results may give an indication of risk of recurrence and influence treatment, as is the case for any patient undergoing evaluation for thrombophilia involving VTE. More detail is available in recent clinical guidelines. 8-10 | Sample handlingVenous blood should be collected into a one-tenth volume of 3.2% (0.105-0.109 mol/L) trisodium citrate, and double-centrifuged to ensure a residual platelet count of <10.0 × 10 9 /L. 4,11,12 As some other thrombophilia assays also require similarly effective platelet removal, this permits running of multiple assays with the same, suitably prepared, plasma sample. The white cells remaining after plasma removal can be stored for DNA extraction should molecular analysis be required, or cells from an EDTA-anticoagulated sample can be used.Plasma for APC-R assays should be tested within 4 hours of collection or frozen (at -20°C if stored for ≤2 weeks, and at −70°C or below if stored for >2 weeks) if testing is postponed. Frozen samples should be rapidly thawed in a waterbath at 37°C, and thoroughly mixed by multiple, gentle inversions prior to testing. Icterus, hemolysis and lipemia can interfere, especially in assays performed on undiluted plasma. Plasma predilution assays are less affected by platelet contamination. 3 Preliminary coagulation screening is useful to detect previously unknown factor deficiencies and anticoagulation, and, if a suitably sensitive APTT reagent is employed, lupus anticoagulants (LAs) may also be detected. | InterferencesAssay design and reag...

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“…Analysis of proficiency testing from DGKL (a proficiency program based in Germany which includes ECAT and NASCOLA laboratories in Europe and North America) shows that molecular testing for factor V Leiden and prothrombin G20210A is very accurate, in that in 2008 all 400 prothrombin G20210A results were correct and 405/406 factor V Leiden results were correct. When errors occurred, many appeared to be transcription or specimen switching errors, because when heterozygous and wild type specimens are sent in the same proficiency test shipment, the error rate was higher [10].…”

Section: Introductionmentioning

confidence: 99%

Advances in laboratory testing for thrombophilia

2012

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Testing for hereditary thrombophilia typically includes tests for activated protein C resistance (APC‐R) and/or factor V Leiden, protein C, protein S, antithrombin, and prothrombin G20210A. New options for these assays have become available in recent years, with different advantages and disadvantages among the currently available methods. Potential interferences for each assay type are discussed, including lupus anticoagulants, heparin, warfarin, direct thrombin inhibitors (such as argatroban, dabigatran, hirudin, or bivalirudin), rivaroxaban, factor deficiencies or elevations, factor V Leiden, and specific mutations that the assay(s) might not be able to detect. Causes of acquired deficiencies are also described, as these must be carefully excluded before diagnosing a hereditary deficiency of protein C, protein S, or antithrombin. Am. J. Hematol. 2012. © 2012 Wiley Periodicals, Inc.

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All that glitters is gold?

Cited by 5 publications

References 12 publications

Factor VLeiden

Factor VLeiden

Recommendations for clinical laboratory testing of activated protein C resistance; communication from the SSC of the ISTH

Advances in laboratory testing for thrombophilia

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