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Stability of Zika virus in urine: Specimen processing considerations and implications for the detection of RNA targets in urine.

Author information

Affiliations

  • 1. Department of Medicine, Division of Infectious Diseases and Geographic Medicine, Stanford University School of Medicine, Stanford, CA, USA.
      Authors
    • Tan SK 1
    (1 author)
  • 2. Department of Pathology, Stanford University School of Medicine, Stanford, CA, USA.
      Authors
    • Sahoo MK 2
    (1 author)
  • 3. Clinical Virology Laboratory, Stanford Health Care, Stanford, CA, USA.
      Authors
    • Milligan SB 3
    • Taylor N 3
    (2 authors)
  • 4. Department of Medicine, Division of Infectious Diseases and Geographic Medicine, Stanford University School of Medicine, Stanford, CA, USA; Department of Pathology, Stanford University School of Medicine, Stanford, CA, USA; Clinical Virology Laboratory, Stanford Health Care, Stanford, CA, USA.
      Authors
    • Pinsky BA 4
    (1 author)

ORCIDs linked to this article

Journal of Virological Methods, 01 May 2017, 248:66-70
https://doi.org/10.1016/j.jviromet.2017.04.018 PMID: 28472623 

Abstract 

Background

Detection of Zika virus (ZIKV) RNA in urine is of increasing interest for the diagnosis of ZIKV infection. Pre-analytical variables can significantly impact the stability of RNA in urine.

Methods

To determine optimal specimen processing protocols that would maximize detection of ZIKV RNA in urine by real-time, reverse transcriptase PCR, we investigated the effect of temperature, initial ZIKV concentration, use of nucleic acid stabilizers, and time on ZIKV RNA levels. Urine samples from healthy donors were spiked with ZIKV using the Exact Diagnostics® ZIKV Verification Panel, a commercially available panel composed of heat-inactivated ZIKV, at concentrations of 5.0 log10 copies/mL (ZIKV-high) and 4.0 log10 copies/mL (ZIKV-low). Samples were stored at room temperature, 4°C, or -80°C and frozen aliquots were exposed to no stabilizer (urine), Buffer ATL (Qiagen, Germantown, MD), or DNA/RNA Shield (Zymo Research, Irvine, CA).

Results

ZIKV RNA levels in urine declined steadily at room temperature, though was not significant by 48h (ZIKV-high, p=0.09; ZIKV-low, p=0.20). ZIKV RNA titers were consistently higher when stored at 4°C, suggesting that storage at 4°C can slow the progression of RNA degradation. Freezing urine samples at -80°C resulted in a significant loss of detectable ZIKV RNA in the ZIKV-low group. ZIKV RNA was detected in 5/6 replicates at 3days, 1/6 replicates at 10days, and 1/3 replicates at 30days, with findings reproducible on repeat testing. Presence of either nucleic acid stabilizer in urine corrected this effect, and resulted in recovery of ZIKV RNA in all replicates. Use of a nucleic acid stabilizer in the ZIKV-high group did not add incremental benefit for the detection or quantitation of ZIKV RNA.

Conclusions

ZIKV RNA is prone to degradation in urine with loss of detectable virus even when specimens are frozen at -80°C for 10days. Detection of ZIKV-positive urine samples, particularly those containing low ZIKV titers may be aided with the addition of a nucleic acid stabilizer during urine specimen processing.

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Read article at publisher's site: https://doi.org/10.1016/j.jviromet.2017.04.018

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Funding 

Funders who supported this work.

NCATS NIH HHS (1)

National Institutes of Health (1)

Stanford Translational Research and Applied Medicine (TRAM) Pilot Grant Program

    TL1 Clinical Research Training Program of the Stanford Clinical and Translational Science Award to Spectrum (1)