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Continuing Studies of Viruses in Hampton Roads and Shellfish

Continuing Studies of Viruses in Hampton Roads and Shellfish Howard Kator, Kimberly Reece, Corinne Audemard, Wendi Ribiero, Martha Rhodes With support from: Hampton Roads District Commission NOAA Sea Grant Virginia Institute of Marine Science. SETTING THE STAGE:

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Continuing Studies of Viruses in Hampton Roads and Shellfish

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  1. Continuing Studies of Viruses in Hampton Roads and Shellfish Howard Kator, Kimberly Reece, Corinne Audemard, Wendi Ribiero, Martha Rhodes With support from: Hampton Roads District Commission NOAA Sea Grant Virginia Institute of Marine Science

  2. SETTING THE STAGE: PREVIOUS WORK REPORTED AT THE LAST ISS MEETING IN VIRGINIA BEACH

  3. VIMS/VDH/VMRC andHRSD Combined Hampton Roads Clam Study

  4. Background • In 2005 the Division of Shellfish Sanitation (DSS), approached VIMS with regard to evaluating the sanitary quality of the Hampton Roads clam (Mercenaria mercenaria) resource. • Specifically, although much of the area is closed to direct harvesting, questions arose concerning the safety of clams harvested from these waters for relay to approved waters for marketing. • VDH concerns centered on the presence of effluents from four waste water treatment plants (WWTP) discharging to the waters of Hampton Roads. • WWTP effluents have been shown to be potential sources of pathogenic human enteroviruses (e. g., van den Berg et al. 2005) and the effectiveness of the relaying process for elimination of viruses such as norovirus (NoV) from clams is unknown.

  5. Background • A Fall 2007 VIMS/VDH study design involved placement of on-bottom cages containing clams at two locations in Hampton Roads followed by analysis of microbial burdens that included NoV, FRNA coliphage and fecal coliforms/Escherichiacoli. • Two locations were chosen on the basis of proximity to the HRSD Nansemond WWTP outfall. • Exposure studies were conducted (Fall 2007) when viral persistence or occurrence would be favored, i. e., in the fall when water temperatures were decreasing.

  6. Figure 1. Location of clam exposure sites for Fall 2007 samples. CLAMS OUTSIDE WWTP BUFFER ZONE CLAMS WITHIN WWTP BUFFER ZONE NANSEMOND WWTP OUTFALL

  7. Table 1. VIMS microbiological results for clams exposed for ca. 2 weeks at the Nansemond WWTP outfall and Condemnation Line 1 ("Cond 1") in Hampton Roads. Samples retrieved and analyzed Nov. 28, 2007.* Clams were sourced from a commercial dealer (Cherrystone Aquaculture) and approved for human consumption. For some samples that were positive for NoV the PCR amplification products were sequenced to determine whether genogroup I, II or both were detected. Detected norovirus on both "sides" of line FRNA coliphage higher near outfall • *Fecal coliforms and E. coli densities determined using the APHA 5-tube MPN with EC-MUG as the medium. FRNA coliphage measured following a proposed FDA method but using Salmonella typhimurium WG49 as the assay host. NoV occurrence indicated as ratio of analytical replicates that were positive by real-time PCR. Water samples collected at the time of shellfish retrieval: • "Cond 1" - <1.8 fecal coliforms and E. coli per 100 ml; <1 FRNA phage per 100 ml; 22.8 psu, 12.1C • Nansemond WWTP outfall - 2.0 fecal coliforms and E. coli per 100 ml; <1 FRNA phage per 100 ml; 22.6 psu, 11.8C.

  8. Table 2. VIMS microbiological results for clams exposed for ca. 3 weeks at the Nansemond WWTP outfall and Condemnation Line 1 (Cond 1) in Hampton Roads. Samples retrieved and analyzed Dec. 4, 2007.* Clams were sourced from a commercial dealer (Cherrystone Aquaculture) and approved for human consumption. Detected norovirus on both "sides" of line FRNA coliphage higher near outfall *Fecal coliforms and E. coli densities determined using the APHA 5-tube MPN with EC-MUG as the medium. FRNA coliphage measured following a proposed FDA method but using Salmonella typhimurium WG49 as the assay host. NoV occurrence indicated as ratio of analytical replicates that were positive by nested PCR. Water samples collected at the time of shellfish retrieval: Cond 1 – 2.0 fecal coliforms and E. coli per 100 ml; <1 FRNA phage per 100 ml; 23.1 psu, 10.1°C Nansemond WWTP outfall - <1.8 fecal coliforms and E. coli per 100 ml; <1 FRNA phage per 100 ml; 22.5 psu, 9.9°C

  9. Figure 2. Clam deployment sites and WWTP effluent locations- Spring 2008 experiments

  10. Figure 2. Clam deployment sites and WWTP effluent locations- Spring 2008 experiments GI GI GI GI GI GII Effluents- GI GII

  11. DNA sequences from sequencing the PCR fragment amplified with GI specific primers and probe. Note the relatively highly conserved sequences with a few nucleotide differences suggesting that there is some genetic strain variation both within and between sites.

  12. 2009 COMPARATIVE RELAY STUDY Contamination under natural conditions Relay into approved waters Crassostrea virginica Mercenaria mercenaria Detect and relate norovirus to FRNA coliphage, measure virus elimination kinetics

  13. 2009- A "strange" year for obtaining shellfish contaminated with norovirus?

  14. Objective: norovirus and FRNA coliphage uptake at densities high enough to follow elimination kinetics over 14 day time course

  15. Cont'd

  16. Cont'd

  17. Cont'd

  18. *Detection of norovirus GI/GII in 2 qPCR analytical replicates of post-chlorinated effluent

  19. Plan one more set of experiments for the Fall of 2010 Either in situ contamination or tank contamination with relay in approved waters? Evaluate virus recovery using APHA 10-12 oyster homogenate versus homogenizing digestive diverticula from 1, 3 or 5 oyster samples to improve detection

  20. VIRUS DETECTION METHODS

  21. Shellfish sample processing for norovirus(based on Jothikumar et al. 2005; Gentry et al. 2009) Homogenization of clam tissues Aliquot 1.5 g (can freeze at this point) Add Buffer + Proteinase K Virus release from the shellfish tissues 37°C for 1 hr with shaking 65°C for 15 min Centrifuge 3000 x g for 5 min, collect supernatant RNA extraction RNA extraction using the MagMAX kit Reverse transcription to obtain cDNA Virus detection qPCR for the detection of GI and for GII DNA sequencing to identify the strain(s) detected

  22. Adenovirus Qualities supporting its evaluation as a candidate indicator: Appears to be stable in aqueous environments Resistant to UV radiation, chlorination Doesn’t appear to have substantial seasonal variation (as does norovirus) Unlike norovirus it can be cultured to address the question of viral infectivity when recovered from the environment

  23. Shellfish sample processing for adenovirus(based on Woods (2006), Puig et al. (1994), and Heim et al. (2003)) Homogenization of clam tissues (can freeze at this point) Adjust conductivity to below 2,000 μS/cm Adjust pH to 4.8, centrifuge to pellet Resuspend pellet in glycine/NaCl, adjust pH to 7.5, centrifuge to pellet Virus release from the shellfish tissues Resuspend pellet in threonine/NaCl, centrifuge to pellet, collect supernatant PEG 8000 precipitation, centrifuge to pellet, resuspend in 1X TE DNA extraction using DNeasy tissue kit DNA extraction qPCR and nested PCR for all strains of human adenovirus Virus detection DNA sequencing to identify the strain(s) detected

  24. Effluent sample processing for norovirus and adenovirus(based on Katayama et al. 2002) Effluent sample + 25mM MgCl2 Adsorption of the virus to a membrane Filter through negatively charged membrane filter (0.45µm) Rinse out cations with H2SO4 Elution of the virus Elute the virus with NaOH Neutralize filtrate with H2SO4 and 100X TE Virus concentration Concentrate using Vivaspin 6 ultrafilter RNA extraction using MagMAX DNA extraction using DNeasy tissue Kit Virus detection Reverse transcription qPCR Nested PCR Automated DNA sequencing qPCR for the detection of GI and for GII

  25. Combined FDA/HRSD/VDH Dye Study of Menchville HRSD Waste Water Treatment Plant-James River Virginia

  26. VIMS participation: (1) Provide a second, independent analysis of oyster (Crassostrea virginica) and effluent samples for indicator and virus presence for HRSD (2) Allow for comparison of results using different viral detection methods.

  27. Parameters to be measured in oysters: Fecal coliforms Escherichia coli FRNA male-specific coliphage Norovirus (strains GI and GII) Adenovirus (human-specific primer set) Parameters to be measured in WWTP samples: Norovirus (strains GI and GII) Adenovirus (human-specific primer set)

  28. Norovirus and human adenovirus in HRSD James River WWTP samples taken during FDA dye release and exposure of sentinel shellfish

  29. Norovirus and human adenovirus in sentinel oysters deployed in the James River during the FDA dye release: first exposure study (4/13/2010 - 4/27/2010)

  30. Norovirus and human adenovirus in sentinel oysters deployed in the James River during the FDA dye release: second exposure study (4/27/2010 - 5/11/2010)

  31. FDA deployed oyster cages +

  32. Outfall FRNA 1 NoV AdV 2 3 4 NoV AdV 5 NoV AdV

  33. Location of "control" sites in Burwell Bay

  34. Proposed Future Work NOAA- Evaluation of conventional and an innovative immunomagnetic method for detecting and monitoring pathogenic human norovirus in bivalve shellfish "….. improving the sensitivity of norovirus detection….." Evaluate adenovirus as a viral indicator

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