Cystic Fibrosis Kit

xTAG® Cystic Fibrosis 39 Kit v2 (USA/Europe)

xTAG® Cystic Fibrosis 71 Kit v2 (Europe)

The xTAG® Cystic Fibrosis 39 Kit v2* and the xTAG® Cystic Fibrosis 71 Kit v2** are uniquely designed to offer physicians the ability to select the CFTR gene mutations for which they want to test. They can select to test a patient for the panel of 23 CFTR gene mutations and 4 variants recommended by the American College of Medical Genetics (AMCG) and American College of Obstetricians and Gynecologists (ACOG), or the entire xTAG® panel of 39 or 71 CFTR gene mutations.

These assays are qualitative genotyping tests which provides information intended to be used for carrier testing in adults of reproductive age, as an aid in newborn screening, and in confirmatory diagnostic testing in newborns and children.

*For In-Vitro use only (510K) cleared and CE Marked.

**For In-Vitro use only CE Marked.

Products listed are region specific and intended for residents of a particular country/region; this site contains information on devices that may not be approved in some countries/regions, therefore please contact Luminex to obtain the appropriate product info for your country of residence.

Benefits:

Confidence:
Second generation of IVD assay >99.9% Precision and Reproducibility.

Comprehensive:
Most comprehensive mutation coverage, including ACMG/ACOG recommended panel.

Flexibility:
Mutation panel selection through the software.

Ease to Use:
Streamlined protocol with minimal hands-on time.

Cost-Effective Multiplex Genotyping:
Reduced repeat rate No reflex testing is necessary.

xTAG® Cystic Fibrosis Assay Technology

Step 1 - Nucleic Acid Extraction and Purification Many commercially DNA extraction kits are available which will provide high quality genomic DNA (UV 260/280 ratios: >1.5-1.7) compatible with the xTAG Cystic Fibrosis 39 kit v2 from human blood specimens. A optimal input quantity of 50ng (range of 10ng to 1.5ug) per sample is required to perform the assay. Step time will vary depending the choice of extraction method.
Step 2 - Multiplex PCR Reaction The nucleic acid is amplified using one polymerase chain reaction (PCR), a molecular biology technique for rapidly creating multiple copies of DNA. In this case, the technique will make multiple copies of multiple DNA target.
Step 3 - Allele-specific primer extension (for CF) The amplified DNA is mixed with short sequences (TAG primers) of DNA specific to each target. If the target is present, the primer will bind and will be lengthened through a process called Allele specific amplification. During this extension, a reporter label is incorporated.
Step 4 - Bead Hybridization Color-coded beads are added to identify the tagged primers. Attached to each differently colored bead is an anti-TAG sequence specific to one of the extended TAG primers. Each anti-TAG only binds to the complementary TAG sequence on the primer.
Step 5 - Addition of Reporter Molecule The reporter solution is the Streptavidin, R-Phycoerythrin conjugate and will be used to detect the target.
Step 6 - Data Acquisition on Luminex Analyser Samples are then placed in a Luminex xMAP® instrument where beads are read and analyzed by lasers. The lasers identify the color of the bead and the presence or absence of the labeled target. For each sample, these signals are interpreted by the xTAG® Data Analysis Software to determine whether the wild-type and/or mutant alleles for each of the variations have been detected.

xTAG® Cystic Fibrosis 39 kit v2 Components

xTAG® Cystic Fibrosis 71 kit v2 Components

DOCUMENTS

Elenco Prodotti

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