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BRUCELLA

BRUCELLA. Main species. Brucella melintensis Brucella abortus Brucella suis. Normal habitat. Obligate intracellular pathogens of animals B. melitensis mainly found in goat and sheep B. abotus infects cattle B. suis found in pigs and occasionally in goat

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BRUCELLA

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  1. BRUCELLA

  2. Main species • Brucella melintensis • Brucella abortus • Brucella suis

  3. Normal habitat • Obligate intracellular pathogens of animals • B. melitensismainly found in goat and sheep • B. abotusinfects cattle • B. suisfound in pigs and occasionally in goat • Other animal including horse, camel, eland and wild rodents

  4. Routes of infection • Mosquitoes helps in transfer Brucellafrom animal to human • Also by ingesting unpastuerized milk or milk products, enter damaged skin or eyes, inhaled in airborne particles or aerosols.

  5. Laboratory diagnostics

  6. Microscopic observation • Non-motile • Gram negative • Coccobacili • Show bipolar staining • Rarely found in direct smear from uncultured specimen • On Gram stain they appear as dense clumps of Gram-negativecoccobacilli and are exceedingly difficult to see.

  7. Culture characteristics • Mostly cultured from blood of high fever patient(Brucellosis) • Isolation is extremely rare in chronic brucellosis • In all blood culture, they need carbon dioxide • Blood culture should be kept in 4 – 6 weeks before result as no organisms isolated • To reduce the risk of contamination, use the diphasic medium such as Castaneda or tryptic soy broth or agar • Brucellae are aerobic with enriched of carbon dioxide

  8. Biochemical tests Serology tests • Urease and hydrogen sulphide production • All brucella strains are catalase positive • Possess two antigens called A and M Famous test serum: • Rapid slide agglutination test • Tube agglutination titration test

  9. Serology test • It is crucial to be able to differentiate Brucella from Salmonella which could also be isolated from blood cultures and are Gram-negative. Testing for urease would successfully accomplish the task; as it is positive for the Brucellaand negative for the Salmonella.

  10. HAEMOPHILUS

  11. Medical important species • Haemophilus influenzae • Haemophilus aegyptius • Haemophilus ducreyi

  12. Normal habitat • H.influenzae (mostly non-capsulated strains), H. parainfluenzaeand H.aegyptiusis normal flora of the upper respiratory tract • Infections causing: • Pyogenic meningitis • Acute epiglottitis • Cellulitis, middle ear infection,etc

  13. conjuctivitis

  14. Laboratory diagnosis

  15. microscopy • Small, non-motile, Gram negative rods or coccobacili • Long thread-like form in old csf culture

  16. Microscopic observation

  17. Culture of H.influnzae • H.influenzae grows better in aerobically compare to anaerobically • The optimum temperature for growth 35 – 37oC • The are X and V factor • Both represent in blood agar and permit the culture to grow • H.influenzae and H.aegyptius need X and V factor, H. parainfluenzaeneed V factor and H.ducreyi need X factor

  18. Biochemical tests • Not usually used to identify hemophilus • 6 biovars of H.influenzae are recognized based on the indole, urease and ornithinedecarboxylase (ODC) reactions of the diff strains

  19. serology • Consist of 1 – f serotypes • Mostly causing meningitis belong to serogroup b • Most strains that cause chronic bronchial disease are non-capsulated Antimicrobial sensitivity • Resistant towards chloramphenicol, ampicilin, tetracycline, erythromycin and cotrimoxazole • H. ducreyiis sensitive to sulphonamides • Ampicillin resistant are common

  20. STAPHYLOCOCCUS & STREPTOCOCCUS

  21. Staphylococcus Staphylococcus aureus Staphylococcus epidermidis Staphylococcus saprophyticus

  22. introduction • Are microbial flora of the skin, upper respiratory tract and intestinal tract • S.aureus usually cause abscesses, boils, conjuctivitis, pneumonia, septicemia, food poisoning and scalded skin syndrome • S. epidermidis causingbacteraemia • S. saprophyticus causing cystitis and acute urethritis

  23. Laboratory diagnosis Microscopy • Non-motile • Non capsulate • Gram positive cocci • Arrangement single or in pair • Size 1 µm diameter

  24. Culture • Grow well in aerobically and also in present of carbon dioxide • Temperature between 10 – 420C, optimum temperature are between 35 - 370C

  25. S.aureus • Produce yellow to cream in blood and chocolate agar (heated agar) • Occationally produce white 1-2 mm in diameter colonies • Some strain produce beta-hemolytic when grown aerobically • Colonies are slightly raised and easily emulsified on a slide • Non- lactose fermenterin MacConkey agar • Mannitol salt agar is a useful differential and selective agar to identify S.aureus

  26. On blood agar

  27. S.epidermidis • Colony is white • Non hemolytic in blood agar S. saprophyticus • Maybe white or yellow • There are non-hemolytic in BA • Not grow anaerobically • No growth in MacConkey agar

  28. Biochemical reactions S.aureus • DNAse test will be positive for S.aureus but negative in other species • Catalase test will be positive in all staphylococcus but negative in all streptococcus S. epidermidisand S. saprophyticus • Coagulase negative • DNAse negative • Catalase positive

  29. Antimicrobial sensitivity • Erythromycin • Clindamysin • Fucidin • Vancomycin • Many strains of S.aureus are penicillin-resistant • S.epidermidis are more resistant than S.aureus to antibiotics • S. saprophyticus less resistant to antibiotics than S.aureus and S.epidermidis

  30. streptococcus Streptococcus pyogenes Streptococcus agalactiae Enterococci

  31. To be continue..

  32. Explain what happens in the following biochemical tests: i) Indole test ii) Methyl red test 8 marks) b) Write the scientific name of a bacterium that gave positive results for both tests. (2 marks)

  33. Question State all group of gram positive and gram negative bacteria.

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