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Mycology – Introduction

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Presentation on theme: "Mycology – Introduction"— Presentation transcript:

1 Mycology – Introduction
Student Lab Division of Medical Technology Carol Larson MSEd, MT(ASCP)

2 Mycoses Superficial Subcutaneous Systemic Opportunistic

3 Characteristics of fungi
Eukaryotic Growth requirements Forms Mold Yeast

4 Hyphae Septate Aseptate

5 Hyphae Hyaline Dematiaceous

6 Mycelium Mass of branching intertwined hyphae Vegetative Aerial
Fertile

7 Vegetative types Favic chandeliers Nodular organs Racquet hyphae
Spiral hyphae

8 Reproduction Identify fungi by: Morphology of reproductive structures
Spores from vegetative mycelium or aerial fruiting bodies

9 Asexual Reproduction Conidia Conidiophore Arthroconidia

10 Asexual Reproduction Blastoconidia Pseudohyphae Chlamydoconidia
Chlamydospores

11 Asexual Reproduction Macroconidia Microconidia Phialoconidia Phialide

12 Asexual Reproduction Annelloconidia Annellide Sporangiospores
Sporangium Sporangiophore

13 Sexual Reproduction Perfect Fungi – has a sexual stage
Fungi Imperfecti – no know sexual stage Spores

14 Sexual Reproduction Ascospores Ascus Ascocarp Basidiospores Zygospores

15 In review … Mycoses – fungal diseases Characteristics of fungi
Growth requirements Forms (mold, yeast) Structures Reproduction Asexual Sexual

16 Fungal Culture Process
Specimen collection and transportation Direct examination of specimen Selection and inoculation of media Evaluation of fungal growth Serological testing Antifungal susceptibility testing

17 Specimen Collection Specimen types
Collect from area most likely infected Use sterile technique Keep specimen moist Label container properly Transport right away Process right away

18 Direct Examination Provides preliminary report
Guides MD in treatment of patient Observe yeast phase of dimorphic Gives clues to id causative agent Inoculate special media May require more than one direct examination method

19 Direct Examination Saline wet mount Lactophenol cotton blue wet mount
10% KOH preparation Gram stain Acid fast stain India ink stain

20 Direct Examination Calcofluor white stain Wright’s stain
Gomori Methenamine Silver stain Periodic Acid Schiff stain

21 Specimen Processing Safety Tube media preferred over plate media
Work in safety hood Wear gloves and lab coat Autoclave specimens and media Disinfect work area daily

22 Specimen Processing Primary isolation media
Goal: isolate potential pathogens Use non-selective and selective media Proper ingredients Incubation temperature Incubation time Incubation atmosphere

23 Non-selective Media Sabouraud dextrose agar
Brain heart infusion (BHI) with/without 5% blood and 1% glucose

24 Selective Media Mycosel agar Inhibitory mold agar
Dermatophyte test medium

25 Subculture / Identification Media
Neutral Sabouraud dextrose agar (Emmon’s) Cornmeal-Tween 80 agar Niger seed agar (Birdseed agar) Tween 80 / Oxgall / caffeic acid agar Potato dextrose agar

26 Examination of Culture Growth
Potential pathogens Slow growers Growth on Mycosel Color: dull buff, brown, mousy gray Dimorphic

27 Examination of Culture Growth
Growth rate Rapid growers: 1-5 days Intermediate growers: days Slow growers: >10 days

28 Colony Morphology – Appearance
Rugose Umbonate Verrucose Flat

29 Colony Morphology – Texture
Cottony Glabrous Granular Velvety

30 Colony Morphology – Pigmentation
Surface Reverse

31 Microscopic Morphology
Definitive means of identification Evaluate: Shape Method of production Arrangement of conidia/spores Size and color of hyphae

32 Microscopic Techniques
Tease mount Scotch tape preparation Slide culture

33 Serological Diagnosis
Immunodiffusion Complement fixation EIA Latex agglutination

34 Antifungal Susceptibility
Determine appropriateness Standardization of testing Methods Predictability in vivo Antifungal agents

35 In Summary … Specimen collection and transport
Specimen processing and culture Direct examination of specimen Examination of culture Serological testing Antifungal susceptibility


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