Order Code MEASR Measles Virus, Molecular Detection, PCR, Throat
Ordering Guidance
Polymerase chain reaction testing (this test) is recommended as the first-line test if a patient has symptoms of measles (ie, cough, fever, conjunctivitis, rash).
If serology has been performed and IgM-class antibodies against measles are detected (ROGM / Measles (Rubeola) Virus Antibody, IgM and IgG, Serum), this test should be ordered to confirm measles infection.
Shipping Instructions
Specimens should be transported as soon as possible.
Specimen Required
Specimen Type: Throat Swab
Supplies: Culturette (BBL Culture Swab) (T092)
Container/Tube: Sterile container with transport media
Specimen Volume: Entire collection
Collection Instructions:
1. Collect specimen by swabbing back and forth over mucosal surface to maximize recovery of cells.
2. Swab must be placed into viral transport media (eg, M4-RT, M4, M5, Bartels FlexTrans Transport Media, Jiangsu Transport Media)
Useful For
Identifying measles virus infection using throat swab specimens
Method Name
Real-Time Polymerase Chain Reaction (PCR)
Reporting Name
Measles Virus PCR, ThroatSpecimen Type
VariesSpecimen Minimum Volume
0.3 mL
Specimen Stability Information
Specimen Type | Temperature | Time | Special Container |
---|---|---|---|
Varies | Refrigerated (preferred) | 7 days | |
Frozen | 7 days |
Reject Due To
E-swab, calcium alginate-tipped swab, wood swab, dry swab, or transport swab containing gel or charcoal additive | Reject |
Reference Values
Negative
Method Description
The measles virus laboratory-developed reverse-transcription polymerase chain reaction (RT-PCR) assay is designed for the qualitative detection of measles virus RNA from urine and throat swabs of patients with suspected infection. Measles virus RNA in clinical specimens is first extracted using the NucliSENS easyMag/EMAG (bioMerieux) instruments according to manufacturer instructions. As a component of extraction, a lysis buffer is first added to clinical specimens in a class II biosafety cabinet (BSC). At this step, any measles virus present in the sample is inactivated, rendering it noninfectious. Following the addition of lysis buffer, specimens are safe to remove from the BSC and placed onto an instrument for automated extraction. A sample input of 200 mcL will be extracted with an elution volume of 50 mcL.
This assay employs a reverse transcription reaction to convert RNA to complementary DNA. Oligonucleotide forward and reverse primers specific to the nucleoprotein (N) gene region of the measles virus amplify the target sequence. A TaqMan probe labeled with the fluorophore FAM and specific to the target region of measles virus RNA binds to amplified measles RNA virus product. Ribonuclease P (RNase P) is used as an internal control. Oligonucleotide forward and reverse primers specific to the p30 subunit of RNase P amplify the internal control target sequence. A TaqMan probe labeled with fluorophore Cy5 and specific to RNase P bind to the amplified RNase P product. The dye-labeled TaqMan probes allow for the detection of the target and internal control in the corresponding channels of the Roche LightCycler 480 II (LC480) instrument. Detection of the target N gene region indicates the presence of measles virus RNA in the specimen. The clinical validity of RT-PCR for the detection of the N gene of measles virus RNA in urine and throat swabs is well documented in peer-reviewed literature.(Unpublished Mayo method)
Day(s) Performed
Monday through Friday
Performing Laboratory
Mayo Clinic Laboratories in RochesterCPT Code Information
87798