1. RECENT ADVANCES IN �RAPID MICROBIAL �IDENTIFICATION AND �CHARACTERIZATION �TECHNIQUES� Mackenzie Slifierz
Hiu Ching Lai
James Feiner
2. Public Health Emergencies Hurricane Katrina, 2005
At least five level 3 biosafety labs within hurricane zone.
3. Public Health Emergencies Hurricane Ike, 2008
Galveston Nation Labs, a level 4 biosafety lab working with potential bioterrorism pathogens including hantavirus, anthrax, and ebola virus.
4. PRESENTATION OVERVIEW Traditional Detection Methods
Advanced Rapid Detection Methods:
PCR-based Methods
Nanotechnology
Immunoassays
Other Rapid Microbial Methods
General advantages and limitations
Conclusion
5. TRADITIONAL DETECTION METHODS Culturing bacteria: colony morphology, colour, and size.
Staining: Gram stain, spore stain, flagella, cell morphology.
Biochemical analysis: carbohydrate utilization and fermentation.
Inhibition: Bile-salts, antibiotic resistance, dye tolerance.
6. Traditional Detection Methods
7. RAPID DETECTION TECHNIQUES What is a rapid detection technique?
A rapid microbial method (RMM) is any technique which can identify or characterize a microorganism in hours or minutes as opposed to days or weeks.
Some techniques that can be used for rapid analysis:
PCR-based Methods
Nanotechnology
Immunoassays
Spectroscopy
Chromatography
8. PCR-based Methods Rapid Identification and Characterization Techniques
9. PCR: POLYMERASE CHAIN REACTION Amplification of microbial DNA.
Detection only requires very little DNA.
Sample is directly from food/clinical sources.
No Culturing.
Advantages:
Low cost (PCR machine: $500)
Quick assay (3.5 hrs)
10. Real-Time PCR (RT-PCR) estimates the quantity of microorganisms in the sample:
11. Designing Primers
Primers can be designed from broad-range/highly conserved bacterial 16S ribosomal genes.
This allows detection of most bacteria but also species-level identification.
Primers can target genes that encode proteins that differentiate known bacteria.
Further detection from the amplified DNA.
13. DIRECT METHOD Design specific fluorescently labeled oligonucleotide probes to differentiate between microorganisms in the sample:
Specific Species (eg E. coli)
Gram Differentiation
Spore formation
Combine with microarray: allows
for many PCR reactions in a single
rapid procedure.
Quick
Efficient
Automated
15. HRMA: �HIGH-RESOLUTION MELTING ANALYSIS Design three conserved primers for three hypervariable regions (V1, V3, and V6) within the 16S rRNA gene.
Double stranded DNA is “melted” and then binds to a fluorescent dye.
17. Compare combinations of V1, V3, V6:
18. EIMS:�ELECTROSPRAY IONIZATION MASS SPECTROMETRY
Primers designed for conserved bacterial 16S ribosomal genes. DNA is amplified by PCR.
Ionize the amplified DNA for mass spectrometry analysis.
Detect the mass of amplified DNA and compare to a database.
21. DGGE:�DENATURING GRADIENT GEL ELECTROPHORESIS Use specific primers to target a region of the bacterial genome and amplify with PCR.
Amplified DNA is run through a denaturing gel.
Different bacterial DNA has different DGGE patterns due to nucleotide content and the secondary structures formed during partial denaturing.
Can determine genus of unknown microorganisms by comparing known DGGE profile.
(eg. Nitrosomonas which oxidizes NH3)
22. Lactobacillus Bacteroides
23. Nanotechnology Rapid Identification and Characterization Techniques
24. NANOTECHNOLOGY Nanotechnology is the creation and manipulation of
matter at the nanoscale.
Nano-constructs capable of self-assembly and specific activity: imitation of natural molecular structures.
Extreme sensitivity reduces
needed sample size.
25. Self-propelled microtubes:
capture-and-release bacteria.
8 um long; 0.5 um diameter.
300 body-lengths/second.
Microengine: platinum-catalyzed oxidation of H2O2 fuel.
Lectin receptor selectively bind bacterial polysaccharides.
Lectin-bacterial bond broken by low-pH gylcine solution.
Mass production: membrane template electrodepostion.
Nanorockets are inexpensive and reusable.
NANOROCKETS
26. Rapid capture and isolation of pathogenic bacteria in complex media.
Duel action: magnetic attachment and release of therapeutic molecules.
H2O2 fuel makes bacteria non-cultural but they remain viable and thus testable.
Biochips: nanorockets scour samples for pathogens in microfluidic channels.
NANOROCKETS
27. SURFACE-ENHANCED-RAMAN-SCATTERING Raman spectroscopy:
Viruses bound to Ag substrate.
Exposed to an infrared laser.
Laser scattered by viral particles.
Spectrograph records signal.
Virus spectral barcodes made.
Silver nanorod substrate:
Enhances spectra cross section by orders of magnitude.
Oblique angle deposition: cheap and simple procedure.
Deposits nanorods in random arrays at an uniform angle.
28. Three strains of the influenza virus (flu):
Each share conserved spectra due to close relation.
Highlighted: non-conserved spectra correlate to variable nucleic acids and surface proteins.
Fast method for detection and classification of viruses, bacteria or toxins.
Monitoring of pollutants.
SURFACE-ENHANCED-RAMAN-SCATTERING
29. CANTILEVERS Cantilevers are horizontal
beams anchored on one end:
Mass bends the cantilever downwards.
A counterbalancing force can restore the original position, resulting in a certain resonance frequency.
The resonance frequency is determined electronically.
Cantilevers can be manufactured at the nanoscale:
Made in dimensions as small as: 5 um x 2 um x 30 nm.
Antibodies attached to cantilevers can detect the binding of single viral or bacterial particles.
Ideal for airborne virus detection or microfluidic biochips.
30. Cantilevers and Atomic
Force Microscopy (AFM):
A nano-pin attached to a cantilever traces cell surfaces.
Pin-cantilever movement is detected by laser deflection.
Produces detailed high resolution topological images of cells and profiles of molecular bond strength.
Rapid microbial detection applications:
Imaging completed in minutes: location of cell-surface markers.
Capable of analyses in aqueous solutions and in vivo.
CANTILEVERS
31.
OmpF: a porin protein of E. coli’s outer membrane:
Forms channels composed of ß – strands (circled).
Left: X-ray crystallography image.
Right: AFM image made with constant force microscopy.
Scale bar: 50 Å. CANTILEVERS
32.
AFM image of a Saccharomyces cerevisiae yeast cell trapped in a microporous membrane, scale: 1 um. CANTILEVERS
33. Force spectrometry on a typical bacterial cell:
Left: a cantilever attached to a membrane polysaccharide encounters resistance as it pulls away from the molecule.
Right: corresponding force-extension curve shows the growing molecular force offered by the polysaccharide as it is stretched. CANTILEVERS
34. IMMUNOASSAYS Rapid Identification and Characterization Techniques
35. IMMUNOASSAYS:�RAPID QUANTIFICATION OF FOODBORNE PATHOGENS Multiplex immunoflourescent technique:
Antibody-Antigen interaction provides specificity and the conjugated flourescent quantum dots allow for rapid detection of multiple pathogens.
36. Quantum Dots
38. Results
39. IMMUNOFLOURESCENT ASSAY Can quantify the number of microorganisms
Relatively quick (< 2 hrs)
Simultaneous detection of multiple microorganisms
Does not require culturing
Sensitive and specific
Expensive
Current methods require technical expertise
Requires lab equipment, but there is a potential for portable equipment
Advantages Disadvantages
40. Immunoassays:�Dipstick Assay for HIV-1 and HIV-2 SD Bioline HIV-1/2 3.0 Test
One step, rapid, immunochromatographic test that can distinguish between HIV-1 and HIV-2, and can detect all isoforms of each!
Sample: human serum/plasma (10 microliter sample) or whole blood (20 microliter sample).
Evaluated by WHO: 99.3% specificity, 100% sensitivity
Time to run test: 5-20 minutes
Price per test: $0.85 – 1.10 USD
42. Direct Sandwich ELISA
43. Results
44. DIPSTICK IMMUNOASSAYS Relatively cheap
Rapid results
Requires very little sample
Very specific and sensitive
Stable over broad temperature range
Easy to transport
Does not require technical expertise to use Qualitative only
Invasive procedure
Disposal
Accidental infections Advantages Disadvantages
45. IMMUNOASSAYS:�USING CHEWING GUM TO DETECT MALARIA Researchers at UCLA have received funding from the Bill and Melinda Gates Foundation to develop an innovative way to detect malaria using chewing gum (MALiVA).
The technique: chewing gum containing antibodies detects malaria-specific antigens in the saliva. The gum is then blotted onto a paper to give a visual result.
This method will be ideal for undeveloped countries where electrical lab equipment and technical expertise is not readily available.
46. Other Rapid Microbial Methods Rapid Identification and Characterization Techniques
47. Computational Analysis and Databases The use of computational analysis provides high-throughput results in a short amount of time.
Data can be shared in online databases.
MALDI – TOF Mass Spectrometry
Matrix-Assisted Laser Desorption Ionisation Time-of-Flight
Species-specific mass spectra of peptides, protein, or other organic molecules by mass spectrometry.
48. MALDI – TOF Mass Spectrometry Very common in clinical biology laboratory:
Efficient
(multiple samples per run)
Cost-effective
($1.80 USD/sample)
Rapid
(<10mins)
49. FAME:�FATTY ACID METHYL ESTER
Cellular fatty acid analysis by Gas Chromatography.
MIDI Sherlock Microbial Identification System.
Comparing fatty acid components to database.
52. Conclusion Rapid Identification and Characterization Techniques
53. Overall Advantages and Disadvantages of �Rapid Microbial Methods: Results are rapid!
Ease-of-use testing.
Tests are made to be very sensitive and specific.
The tests can be portable.
Reduces workload on medical laboratories.
Can test for microorganisms that cannot be cultured.
Allows for earlier detection and faster treatment. Expensive investment in new lab equipment.
May require additional technical expertise.
Potential for abuse: may be used for bioterrorism.
Censorship of scientific data can hinder new developments in this field.
Advantages Disadvantages
54. THE FUTURE! Phasing out of culture-based microscopy:
Can’t compete with superior techniques and
lower cost methods.
Unable to rectify its own flaws.
Take-home diagnosis and treatment kits:
Prepackaged reagents and protocols:
available at your local superstore!
Rapidly identify disease-causing
pathogens and recommend or
provide the appropriate treatment.
Cheap and mass produced, affordable to the developing nations: improvement in global health.
55. QUESTIONS?
