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MICROBIOLOGY RESEARCH AT SOUTHERN CALIFORNIA COASTAL WATER RESEARCH PROJECT (SCCWRP)

MICROBIOLOGY RESEARCH AT SOUTHERN CALIFORNIA COASTAL WATER RESEARCH PROJECT (SCCWRP). Stephen B. Weisberg Executive Director. WHAT IS SCCWRP?. Joint Powers Agency founded in 1969 Initiated to address regional monitoring and research needs Cumulative regional assessments Methods development

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MICROBIOLOGY RESEARCH AT SOUTHERN CALIFORNIA COASTAL WATER RESEARCH PROJECT (SCCWRP)

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  1. MICROBIOLOGY RESEARCH ATSOUTHERN CALIFORNIA COASTAL WATER RESEARCH PROJECT(SCCWRP) Stephen B. WeisbergExecutive Director

  2. WHAT IS SCCWRP? • Joint Powers Agency founded in 1969 • Initiated to address regional monitoring and research needs • Cumulative regional assessments • Methods development • Data integration • Member organizations include city, county, state, and federal agencies • Unique combination of regulators and regulated

  3. MEMBER ORGANIZATIONS • City of San Diego • City of Los Angeles • Ventura County Flood Control District • Los Angeles County Department of Public Works • Los Angeles County Sanitation Districts • Orange County Sanitation District • San Diego Regional Water Quality Board • Santa Ana Regional Water Quality Board • Los Angeles Regional Water Quality Board • State Water Resources Control Board • U.S Environmental Protection Agency

  4. SOME DIFFICULTIES WITH BACTERIAL MONITORING SYSTEMS • Laboratory processing is slow • You should not have been swimming yesterday • Relationship to health risk is not well established • Santa Monica Bay Epidemiology study is the only one to evaluate urban runoff • Poor relationship between bacteria and pathogens • Hard to fix if we don’t know the source • Difficult to define appropriate clean-up levels • Background is not zero

  5. SOME DIFFICULTIES WITH BACTERIAL MONITORING SYSTEMS • Laboratory processing is slow • You should not have been swimming yesterday • Relationship to health risk is not well established • Santa Monica Bay Epidemiology study is the only one to evaluate urban runoff • Poor relationship between bacteria and pathogens • Hard to fix problems if we don’t know the source • Difficult to define appropriate clean-up levels • Background is not zero

  6. SCCWRP’s MICROBIOLOGICAL RESEARCH • Rapid microbiological measurement methods development • Mission Bay epidemiology study • Microbiological source tracking evaluation • Natural sources loading

  7. NEED FOR RAPID MEASUREMENT METHODS • Present methods are slow • Culture-based • Take 24-96 hours • Slow speed compromises the warning system • Exposure occurs during sample processing • Most events last less than 24 hours • Slow speed also compromises upstream tracking • Need a “Geiger counter”

  8. Surface Proteins Small molecules ATP Nucleic Acids Molecules released into medium Things to Measure in a Bacterium

  9. CONCENTRATION TECHNIQUES: IMMUNOMAGNETIC SEPARATION (IMS) Magnetic Beads Antibody Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y = Magnetic Bead Y = Antibody

  10. MIX BEADS WITH ENVIRONMENTAL SAMPLE Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y silica Clay Algae Bacterium Clay Clay Algae

  11. EXPOSE MIXTURE TO MAGNET SYSTEM FOR SEPARATION (E.G. MILTENYI, IMMUNICON OR DYNAL) Add Buffer & Dye Place tube in field Collect Bacteria 30 min. Bacteria move to tube walls Remove Non-magnetic Debris S N N S

  12. FLOW CYTOMETRY: OPTICS Labeled bacterium Scatter Detector Scatter signal Fluorescence Detector Laser excitation Fluorescence signal High performance filters

  13. “Near Real Time Microbial Analysis”

  14. APPROACH • Adapt technology from other industries • Drinking water • Hospital testing • Food service • Counter – bioterrorism • Partner with specialists in these areas • Held a workshop in Monterey in May • Shared developments to date • Defined method evaluation protocols • Will conduct blind testing this summer

  15. MISSION BAY EPIDEMIOLOGY STUDY • Is there a health risk of swimming in Mission Bay? • Comparison of swimmers and non-swimmers • Can we relate to bacterial indicator concentration? • Comparison among swimmers at different times and locations • Can we relate health risk to non-traditional microbiological indicators? • Virus • Phage • Bacteroides

  16. SAMPLING DESIGN • Six beaches • 32 sampling days • Between 2 and 5 sampling sites per beach • Dependent on beach length and swimmer density • Sampled hourly from 12:30 to 3:30 • Total and fecal coliforms by MF • Enterococcus by Idexx • Single beach composite at 12:30 • Phage, virus, Bacteroides • Total and fecal by Idexx • Enterococcus by MF

  17. ENROLLMENT – ACTUAL VS. GOAL

  18. DEMOGRAPHICS OF STUDY POPULATIONRACE AND GENDER

  19. PRIOR LARGE RECREATIONAL WATER STUDIES

  20. SCCWRP’s MICROBIOLOGICAL RESEARCH • Rapid microbiological measurement methods development • Mission Bay epidemiology study • Microbiological source tracking evaluation • Natural sources loading

  21. MICROBIOLOGICAL SOURCE TRACKING • MST tools potentially allow managers to discriminate between human and non-human sources • Some even discriminate among non-human sources • There are more than a dozen proposed MST methods • Most have had limited testing • No marine testing • Which methods are most cost-effective? • How reliable are the results?

  22. STUDY DESIGN • Characterize five sources • Human (direct samples) • Human (sewage influent) • Dog • Cow • Seagull • Place these sources in combination into “blind” water matrix samples • Three matrices • Freshwater • Saltwater • Freshwater with humic acid addition

  23. EXAMPLE TEST MATRIX

  24. STUDY CONCLUSIONS • No method predicted source material perfectly • Genetic techniques did best • Identified dominant sources in about 75% of samples • Phenotypic techniques produced many false positives • Host-specific PCR showed the most promise • Not yet quantitative • Only developed for two sources so far • Viral measures accurately identified sewage, but did not identify individual human sources

  25. NATURAL LOADING PROJECT • Determine properties of waterbodies in undeveloped watersheds • Measure a wide array of constituents • Bacteria • Metals • Nutrients • Provide perspective for various activities • 303D listing • Model calibration • TMDL development

  26. SAMPLING DESIGN • 12 sampling sites • Stratified based on geology and land cover • Dry season sampling • Twice per year (fall and spring) • Two years (2004-2005) • Wet season sampling • Two – three storms at each site • Multiple samples over duration of the storm • Sampled burned vs. unburned catchments twice this winter

  27. Questions or Comments? Steve Weisberg – Southern Ca. Coastal Water Research Project 714-372-9203 stevew@sccwrp.org

  28. SOME TOUGH ISSUES • Measuring low concentrations • Many detectors are based on 1 ml sample • State standard is 104 bacteria per 100 ml • Dead or alive? • Do our standards apply when measuring fragments? • Intercalibration tests are necessary • How do we use real-time information in a patchy environment? • Rapid processing allows adaptive sampling • Lesser processing cost allows more samples • Capital equipment and training costs • Many technologies require up-front investment • Some require specialized training • Per sample cost is typically lower

  29. REPORTED ILLNESSES

  30. COMPARISON TO THRESHOLDS

  31. POTENTIAL TOOLSNATURAL SOURCES IDENTIFICATION • Microbial source tracking – bacteria • Iron-normalization – metals • Chiral chemistry – organics • Compound specific istotope analysis - organics

  32. IRON NORMALIZATION

  33. CHIRAL ENVIRONMENTAL CHEMISTRYENANTIOMERS: MIRROR IMAGES The Ultimate in Pollutant Speciation R-(-) o,p-DDT S-(+) o,p-DDT

  34. COMPOUND SPECIFIC ISOTOPE ANALYSIS • Elements occur in various isotope ratios (e.g. 12C/13C) • IR’s are affected by many natural and anthropogenic processes • Can be extremely effective for source identification

  35. OUR APPROACH • Held a workshop jointly with USEPA to develop method evaluation protocols • Defined four phases of testing • Sequentially increasing level of complexity • Conducted an evaluation test last year • 22 research labs • Tested 12 different MST methods

  36. EXAMPLE MST METHODS • Phenotypic • Antibiotic resistance profiling • Carbon source utilization • Genotypic • Ribotyping • Pulsed field gel electrophoresis • Polymerase chain reaction • Library-independent genotypic • Terminal restriction fragment length polymorphism • Host-specific PCR • Toxin genes • Direct pathogen measurement • Adenovirus • Enterovirus • Phage

  37. EVALUATION CRITERIA • Distinguish presence/absence of human source • Correctly identify all sources • Accurately determine relative contribution from each source • Stability across matrices

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