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Identification methods for oral microbes

Dr. Ali Yaldrum
Dr. Ali Yaldrum

Develop an understanding of Taxonomy (classification) of Oral Microorganisms Describe how to obtain samples from Oral Cavity Describe Molecular techniques of identification Describe techniques that requires culture for identification

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Identification Methods of Oral Microbes Dr. Ali Yaldrum Faculty of Dentistry SEGi University, Kota Damansara, Malaysia 18-06-12
Learning Objectives At the end of this session, the student should be able to: • Develop an understanding of Taxonomy (classification) of Oral Microorganisms • Describe how to obtain samples from Oral Cavity • Describe Molecular techniques of identification • Describe techniques that requires culture for identification
Infection? Virus? culture 2 1 diagnosis Clinician + 3 request treatment 8 What the!!! *A-A-ah Diagnostic interpretation Cycle collection data flow 4 transportation 7 labortary analysis 5 6
VS 1. prokaryotes eukaryotes
prokaroyte cell wall peptidoglycan singular supercoiled circular chromosome flagellum cytoplasm rich in plasmid cellmembrane ribosomes (Fig.1)
eukaroyte mitochondria cell membrane nuclear membrane lysosome cytoplasm rough endoplasmic smooth endoplasmic reticulum reticulum Golgi apparatus (Fig.2)
2. Classification & Identification
classification ‘Classification is the arrangement of Organisms into groups (taxa) on the basis of their similarities and differences.’ The science of classification is called taxonomy
taxonomic hierarchy (Fig.3) KINGDOM PHYLUM DIVISION CLASS ORDER FAMILY GENUS SPECIES SUB SPECIES
identification ‘is the process of determining that a new isolate belongs to particular taxon’ • Bacteria are identified using phenotype, immunological or molecular characteristics
why this is important • Revealing their identity • Behavior and likely response to treatment • Also to predict their pathogenicity • Isolate microorganisms that spread in community & cause serious disease
Bacterial (Fig.4) Classification Shapes Cell wall Outer membrane Teichoic acid protein peptidoglycan Thin Gram peptidoglycan Reaction layer Gram +ve Gram -ve Obligate aerobes requires O2 Plasma membrane Microaerophiles requires reduced O2 Atmosphere Obligate anaerobes requires no O2 Facultative anaerobes anaerobic or aerobic Capnophiles requires increases CO2 Spores Key Enzymes Bacteria lacking certain enzymes Interaction of antibodies with certain Serological Reaction surface structures DNA sequencing of key genes ; Ribosomal 16S gene DNA SEQUENCING
bacterial shapes Coccus Vibrio Bacillus Spirillum Coccobacillus Spirochete Fusiform bacillus (Fig.5)
3. sampling Oral bacteria
• Oral Cavity contains a variety of different niches that harbour distinctive communities of bacteria. • Location and environment determines the diversity of eco system.
Studies of various niches have shown distinctive microbial profiles for different locations • Tongue • Tooth surface • Gingival sulcus • Buccal mucosa • Gingival crevice
gingival sulcus 1 2 3 4 5 6 1= Enamel 4= Free gingivae 2= Dentine 5= Cementum (Fig.6) 3= Pulp 6= Alveolar bone
sampling saliva • Easily sampled • Contains a mix of bacteria (planktonic) • Patient is asked to chew paraffin prior to collecting saliva • Results in enriched tooth derived saliva • Used for collection of large population samples
sampling plaque 2 approaches can be used 1.Supragingival plaque 2.Subgingival plaque
Supragingival • Curette is used to scrap the biofilm of the tooth surface (fig. 7) • Can not be inserted more than 6mm
Periodontal Curette (Fig.7)
Subgingival • Endodontic paper (paper point) can be used (fig. 8) • For pockets deeper than 6mm • Wicks up fluid containing bacteria • Large number of bacteria can be obtained
Endodontic Paper (paper point) (Fig.8)
4. Identifying Oral bacteria
Approaches to identifying bacteria can be grouped into 2major categories • Techniques that do not require culture (molecular identification techniques) • Techniques that require culture *At present combination of both techniques is used to characterize the full compliment of organisms
molecular identification • are most often based on sequence analysis of the ribosomal 16S genes • Common techniques for molecular detection of bacteria: 1. PCR with specific primers 2. Quantitative PCR 3. DNA hybridization assays 4. Ribosomal 16S cloning & sequence analysis 5. FISH and microscopy
bacterial DNA recovery • To extract the bacterial DNA, the bacterial cell wall must be lysed with out damage to the DNA • Several methods are available • Methods that yield high recovery of DNA in one organism might not yield same amount in another
dna recovery COMMERCIAL “KITS’ Detergents Bead Beating & Proteinase K • Target one type of bacteria • Lyse a wide spectrum of • Bacteria are mixed with • Variable intensity bacteria small slurry of tiny glass • High specificity • Unable to lyse Gram-ve beads bacteria • Vile is placed in a vibrating apparatus • Will lyse the most sturdy bacteria's • Not used for fragile bacteria
what is PCR • Or “Polymerase Chain Reaction” ‘It is the process which results in cyclic amplification of target DNA using specific primers, theoretically from one single cell’
what is a Primer The simplest explanation of a primer is to consider it as a “key”, as every key is specific to a particular lock. So every primer is a strand of nucleic acid specific to a specific strand of DNA from a specific specie
what is a Primer ‘A primer is a strand of nucleic acid that serves as a starting point for DNA synthesis. They are required for DNA replication because the enzymes that catalyze this process’ *Primers are usually short, chemically synthesized oligonucleotides, with a length of about twenty bases
PCR • Almost every DNA based method uses PCR • Allows detection of DNA from as low as one cell • Possible to do extensive, detailed analysis • Specific amplification of DNA from a target species even in the presence of hundred of species
variations of PCR The basic PCR methodology is modified to provide sophisticated analytical tools •Nested PCR •Multiplex PCR •Real Time PCR
Real-time PCR • Conventional PCR requires Gel-electrophoresis for amplification analysis • Labelled probes are used • Multiple amplifications can be analysed at specific time period during reaction period
Watch Video of PCR & Gel Electrophoresis https://www.youtube.com/watch?v=GLgt-EGkhZs&feature=related
why is PCR widely used • Even a minuscule quantity of DNA can be studied, as a single DNA molecule is adequate for amplification • Rapid Clinical diagnostic procedures. Sensitivity of PCR enables rapid diagnosis • Enables identification of different species. PCR allowed researcher to identify uncultivable bacteria
DNA Hybridization • Measures the degree of genetic similarity between pools of DNA sequences (fig. 9) • Possible to determine the genetic distance between two sequences • Because of the complexity of bacterial ecology, necessary to identify many species of bacteria from single sample
S. mutans all streptococci Checkerboard hybridization (Fig.9)
Watch video of DNA Hybridization http://www.phgfoundation.org/tutorials/dna/2.html
Watch video of DNA Microarrays http://www.phgfoundation.org/tutorials/dna/6.html
cultivation of bacteria • Consist of diverse group of bacteria • Requires a spectrum of physical & chemical for successful growth • Laboratory cultivation conditions must be adjusted
Bacterial identification process GenusX species 1 species 2 species 3 1 2 3 4 5 Sample & disperse, dilute & plate pick individual characterize by classify transport Onto selective or non colonies & grow morphology & bio- selective media pure cultures chemical tests (Fig.10)
O2 requirements • Amount of O2 in the atmosphere is critical for bacterial growth • Most Oral Bacteria are 1. Facultative anaerobes or 2. Anaerobes 3. Capanophilic anaerobes (A. actinomysetemcomitans)
O2 requirements • Facultative anaerobes a) Streptococcus mutans b) Lactobcillus Both cause caries and can be grown in environment rich in O2
CO2 requirements • Subgingival species are exclusively anaerobic • Must be grown in special chambers containing low levels of CO2 (fig.11) O2 can be removed from the transport medium i. Boiling the media ii. Flushing with O2 free gas iii. Commercially available pre reduced media
Anaerobic Chamber (Fig.11)
culture media Non-selective media • Blood agar supports growth of many oral species • Oral sample will produce diverse array of colony morphologies • Difficult to sort out individual species • Species comprising of small percentage might not be seen
culture media Selective media • Contains ingredients that inhibit growth of all but a few species • Useful in isolating individual species • Enables detection of bacteria that are present in low levels
culture media Special requirements • Some bacteria have specific nutritional requirements • Difficult to grow until those requirements are determined & supplimented
Dispersion & Dilution DNA extraction Non-selective & 16S rRNA gene amplification with Selective agars universal primers Incubate under appropriate Cloning & partial atmospheric conditions sequencing for various times Search for homology Colony count in database Construction of specific Identification scheme probes for subsequent analysis
references • Philip D. Marsh, Michael V Martin, “The Resident Oral Microflora” in Oral Microbiology, 5th Edition, Churchil Livingstone, 2009, pp 24-29 • Philip D. Marsh, Michael V Martin, “Methods of Determining Composition of the resident oral Microflora” in Oral Microbiology, 5th Edition, Churchil Livingstone, 2009, pp 50-54   • Eugene J. Leys, Ann L. Griffen, Purnima S. Kumar and Mark F. Maiden, “Isolation, classification and identification of Oral Microorganisms” in oral Microbiology and Immunology, ASM Press pp 73-88. • PCR - DNA Fingerprinting https://www.youtube.com/watch?v=GLgt-EGkhZs&feature=related • DNA Microaarays http://www.phgfoundation.org/tutorials/dna/6.html • Hybridization http://www.phgfoundation.org/tutorials/dna/2.html • FISH http://www.phgfoundation.org/tutorials/dna/3.html http://www.dnalc.org/view/15924-Making-many-copies-of-DNA.html

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Identification methods for oral microbes

  • 1. Identification Methods of Oral Microbes Dr. Ali Yaldrum Faculty of Dentistry SEGi University, Kota Damansara, Malaysia 18-06-12
  • 2. Learning Objectives At the end of this session, the student should be able to: • Develop an understanding of Taxonomy (classification) of Oral Microorganisms • Describe how to obtain samples from Oral Cavity • Describe Molecular techniques of identification • Describe techniques that requires culture for identification
  • 3. Infection? Virus? culture 2 1 diagnosis Clinician + 3 request treatment 8 What the!!! *A-A-ah Diagnostic interpretation Cycle collection data flow 4 transportation 7 labortary analysis 5 6
  • 5. prokaroyte cell wall peptidoglycan singular supercoiled circular chromosome flagellum cytoplasm rich in plasmid cellmembrane ribosomes (Fig.1)
  • 6. eukaroyte mitochondria cell membrane nuclear membrane lysosome cytoplasm rough endoplasmic smooth endoplasmic reticulum reticulum Golgi apparatus (Fig.2)
  • 7. 2. Classification & Identification
  • 8. classification ‘Classification is the arrangement of Organisms into groups (taxa) on the basis of their similarities and differences.’ The science of classification is called taxonomy
  • 9. taxonomic hierarchy (Fig.3) KINGDOM PHYLUM DIVISION CLASS ORDER FAMILY GENUS SPECIES SUB SPECIES
  • 10. identification ‘is the process of determining that a new isolate belongs to particular taxon’ • Bacteria are identified using phenotype, immunological or molecular characteristics
  • 11. why this is important • Revealing their identity • Behavior and likely response to treatment • Also to predict their pathogenicity • Isolate microorganisms that spread in community & cause serious disease
  • 12. Bacterial (Fig.4) Classification Shapes Cell wall Outer membrane Teichoic acid protein peptidoglycan Thin Gram peptidoglycan Reaction layer Gram +ve Gram -ve Obligate aerobes requires O2 Plasma membrane Microaerophiles requires reduced O2 Atmosphere Obligate anaerobes requires no O2 Facultative anaerobes anaerobic or aerobic Capnophiles requires increases CO2 Spores Key Enzymes Bacteria lacking certain enzymes Interaction of antibodies with certain Serological Reaction surface structures DNA sequencing of key genes ; Ribosomal 16S gene DNA SEQUENCING
  • 13. bacterial shapes Coccus Vibrio Bacillus Spirillum Coccobacillus Spirochete Fusiform bacillus (Fig.5)
  • 14. 3. sampling Oral bacteria
  • 15. • Oral Cavity contains a variety of different niches that harbour distinctive communities of bacteria. • Location and environment determines the diversity of eco system.
  • 16. Studies of various niches have shown distinctive microbial profiles for different locations • Tongue • Tooth surface • Gingival sulcus • Buccal mucosa • Gingival crevice
  • 17. gingival sulcus 1 2 3 4 5 6 1= Enamel 4= Free gingivae 2= Dentine 5= Cementum (Fig.6) 3= Pulp 6= Alveolar bone
  • 18. sampling saliva • Easily sampled • Contains a mix of bacteria (planktonic) • Patient is asked to chew paraffin prior to collecting saliva • Results in enriched tooth derived saliva • Used for collection of large population samples
  • 19. sampling plaque 2 approaches can be used 1.Supragingival plaque 2.Subgingival plaque
  • 20. Supragingival • Curette is used to scrap the biofilm of the tooth surface (fig. 7) • Can not be inserted more than 6mm
  • 22. Subgingival • Endodontic paper (paper point) can be used (fig. 8) • For pockets deeper than 6mm • Wicks up fluid containing bacteria • Large number of bacteria can be obtained
  • 23. Endodontic Paper (paper point) (Fig.8)
  • 24. 4. Identifying Oral bacteria
  • 25. Approaches to identifying bacteria can be grouped into 2major categories • Techniques that do not require culture (molecular identification techniques) • Techniques that require culture *At present combination of both techniques is used to characterize the full compliment of organisms
  • 26. molecular identification • are most often based on sequence analysis of the ribosomal 16S genes • Common techniques for molecular detection of bacteria: 1. PCR with specific primers 2. Quantitative PCR 3. DNA hybridization assays 4. Ribosomal 16S cloning & sequence analysis 5. FISH and microscopy
  • 27. bacterial DNA recovery • To extract the bacterial DNA, the bacterial cell wall must be lysed with out damage to the DNA • Several methods are available • Methods that yield high recovery of DNA in one organism might not yield same amount in another
  • 28. dna recovery COMMERCIAL “KITS’ Detergents Bead Beating & Proteinase K • Target one type of bacteria • Lyse a wide spectrum of • Bacteria are mixed with • Variable intensity bacteria small slurry of tiny glass • High specificity • Unable to lyse Gram-ve beads bacteria • Vile is placed in a vibrating apparatus • Will lyse the most sturdy bacteria's • Not used for fragile bacteria
  • 29. what is PCR • Or “Polymerase Chain Reaction” ‘It is the process which results in cyclic amplification of target DNA using specific primers, theoretically from one single cell’
  • 30. what is a Primer The simplest explanation of a primer is to consider it as a “key”, as every key is specific to a particular lock. So every primer is a strand of nucleic acid specific to a specific strand of DNA from a specific specie
  • 31. what is a Primer ‘A primer is a strand of nucleic acid that serves as a starting point for DNA synthesis. They are required for DNA replication because the enzymes that catalyze this process’ *Primers are usually short, chemically synthesized oligonucleotides, with a length of about twenty bases
  • 32. PCR • Almost every DNA based method uses PCR • Allows detection of DNA from as low as one cell • Possible to do extensive, detailed analysis • Specific amplification of DNA from a target species even in the presence of hundred of species
  • 33. variations of PCR The basic PCR methodology is modified to provide sophisticated analytical tools •Nested PCR •Multiplex PCR •Real Time PCR
  • 34. Real-time PCR • Conventional PCR requires Gel-electrophoresis for amplification analysis • Labelled probes are used • Multiple amplifications can be analysed at specific time period during reaction period
  • 35. Watch Video of PCR & Gel Electrophoresis https://www.youtube.com/watch?v=GLgt-EGkhZs&feature=related
  • 36. why is PCR widely used • Even a minuscule quantity of DNA can be studied, as a single DNA molecule is adequate for amplification • Rapid Clinical diagnostic procedures. Sensitivity of PCR enables rapid diagnosis • Enables identification of different species. PCR allowed researcher to identify uncultivable bacteria
  • 37. DNA Hybridization • Measures the degree of genetic similarity between pools of DNA sequences (fig. 9) • Possible to determine the genetic distance between two sequences • Because of the complexity of bacterial ecology, necessary to identify many species of bacteria from single sample
  • 38. S. mutans all streptococci Checkerboard hybridization (Fig.9)
  • 39. Watch video of DNA Hybridization http://www.phgfoundation.org/tutorials/dna/2.html
  • 40. Watch video of DNA Microarrays http://www.phgfoundation.org/tutorials/dna/6.html
  • 41. cultivation of bacteria • Consist of diverse group of bacteria • Requires a spectrum of physical & chemical for successful growth • Laboratory cultivation conditions must be adjusted
  • 42. Bacterial identification process GenusX species 1 species 2 species 3 1 2 3 4 5 Sample & disperse, dilute & plate pick individual characterize by classify transport Onto selective or non colonies & grow morphology & bio- selective media pure cultures chemical tests (Fig.10)
  • 43. O2 requirements • Amount of O2 in the atmosphere is critical for bacterial growth • Most Oral Bacteria are 1. Facultative anaerobes or 2. Anaerobes 3. Capanophilic anaerobes (A. actinomysetemcomitans)
  • 44. O2 requirements • Facultative anaerobes a) Streptococcus mutans b) Lactobcillus Both cause caries and can be grown in environment rich in O2
  • 45. CO2 requirements • Subgingival species are exclusively anaerobic • Must be grown in special chambers containing low levels of CO2 (fig.11) O2 can be removed from the transport medium i. Boiling the media ii. Flushing with O2 free gas iii. Commercially available pre reduced media
  • 46. Anaerobic Chamber (Fig.11)
  • 47. culture media Non-selective media • Blood agar supports growth of many oral species • Oral sample will produce diverse array of colony morphologies • Difficult to sort out individual species • Species comprising of small percentage might not be seen
  • 48. culture media Selective media • Contains ingredients that inhibit growth of all but a few species • Useful in isolating individual species • Enables detection of bacteria that are present in low levels
  • 49. culture media Special requirements • Some bacteria have specific nutritional requirements • Difficult to grow until those requirements are determined & supplimented
  • 50. Dispersion & Dilution DNA extraction Non-selective & 16S rRNA gene amplification with Selective agars universal primers Incubate under appropriate Cloning & partial atmospheric conditions sequencing for various times Search for homology Colony count in database Construction of specific Identification scheme probes for subsequent analysis
  • 51. references • Philip D. Marsh, Michael V Martin, “The Resident Oral Microflora” in Oral Microbiology, 5th Edition, Churchil Livingstone, 2009, pp 24-29 • Philip D. Marsh, Michael V Martin, “Methods of Determining Composition of the resident oral Microflora” in Oral Microbiology, 5th Edition, Churchil Livingstone, 2009, pp 50-54   • Eugene J. Leys, Ann L. Griffen, Purnima S. Kumar and Mark F. Maiden, “Isolation, classification and identification of Oral Microorganisms” in oral Microbiology and Immunology, ASM Press pp 73-88. • PCR - DNA Fingerprinting https://www.youtube.com/watch?v=GLgt-EGkhZs&feature=related • DNA Microaarays http://www.phgfoundation.org/tutorials/dna/6.html • Hybridization http://www.phgfoundation.org/tutorials/dna/2.html • FISH http://www.phgfoundation.org/tutorials/dna/3.html http://www.dnalc.org/view/15924-Making-many-copies-of-DNA.html