parasitology basic identification methods
TRANSCRIPT
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HUMAN PARASITOLOGY BASIC IDENTIFICATION METHODS
Dr.T.V.Rao MD
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BASIC TERMINOLOGY AND PRINCIPLES
• Symbiosis: Living together
• Commensalism: One symbiont benefits, other unaffected
• Mutualism: Both symbionts benefit
• Parasitism: One symbiont benefits, other is damaged
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The Reality of Parasites
• 1.3 billion persons infected with Ascaris (1: 4 persons on earth)
• 300 million with Schistosomiasis
• 100 million new malaria cases/ year
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Laboratory Methods For Parasites In Faeces
• No technique is 100% successful in detecting parasites by a single stool examination, and at least three serial stools must be examined before a patient can be considered free from infections in which stages of parasites would be expected to be found in the faeces.
• Whilst clinical symptoms or a case history may provide clues as to which parasites may be present, each faecal specimen should be treated as an unknown, as parasite stages unrelated to the clinical picture may be present.
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Faecal specimens may contain several stages of Parasites
• Faecal specimens are examined for the presence of protozoa and helminthes larvae or eggs.
• The stages of protozoa found in stools are trophozoites and cysts. The stages of helminthes usually found in stools are eggs and larvae, though whole adult’s worms or segments of worms may also be seen. Adult worms and segments of tapeworms are usually visible to the naked eye, but eggs, larvae, trophozoites, and cysts can be seen only with the microscope.
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Collection of faecal specimens
1. Because of the fragile nature of many intestinal parasites, and the need to maintain their morphology for accurate identification, reliable microscopic diagnosis can’t be made unless the stool is collected properly.
2. Approximately 10 grams of fresh faeces uncontaminated by urine, oil, water, dyes or radio-opaque into a clean plastic container.
3. The container should be free from antiseptics and disinfectants.
4. Label all samples clearly with the patient’s name, reference number, date, and time of collection.
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Collection of faecal specimens
5. All samples should be accompanied by a requisition form from the physician giving relevant clinical details and recent travel history.
6. Samples and forms from patients with a confirmed or suspected diagnosis of certain infectious diseases such as AIDS or hepatitis should be clearly labeled with “Risk of Infection” or “Biohazard”
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Collection of faecal specimens
• 7.Most viable parasites are susceptible to desiccation or temperature variation. If time lapse between collection and observation is considerable, i.e. more than 4 days, it may be necessary to add some form of preservative to the faeces to retain the morphology as near to the original as possible.
• 8. Formed samples can be kept in a refrigerator at + 4c for a short while, but not in incubator.
• 9. Any whole worms or segments passed should be placed in a separate container
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Collect the Information of the Patient
• History (Age, occupation, residency, previous infection)
• Complaint
• Clinical examination
• Investigations
- Laboratory investigations
- Radiology
- Surgical intervention (Exploratory)
Provisional diagnosis
Confirm the diagnosis
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The Microscopy in Parasitology
• The Microscope is the parasitologist’s main tool. If possible the Microscope- should be binocular; most suitable objectives are the x10, x40, and x100.
• The Microscope must be covered and immersion oil removed from the lens -with xylene or ether when not in use.
• Calibration of the Microscope Eyepiece Micrometer:–On many occasions measuring the size of
suspected parasites in faeces is helpful for identification.(eyepiece micrometer)18-01-2018 Dr.T.V.Rao MD
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Microscopic Examination of Wet Mount
• Wet mount is the simplest and easiest technique for the examination of faeces, and this method should be performed in all laboratories at the peripheral level.
• A wet mount can be prepared directly from faecal material or from concentrated specimens. The basic types of wet mount that should be used for each faecal examination are saline, iodine, and buffered methylene blue.
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The saline wet mount
• Is used for the initial microscopic examination of stools. It is employed primarily to demonstrate worm's eggs, larvae, protozoan trophozoites, and cysts.
• This type of mount can also reveal the presence of red blood cells and white blood cells.
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The Iodine wet mount
• Is used mainly to stain glycogen and the nuclei of cysts, if present. Cysts can usually be specifically identified in this mount.
• The buffered methylene blue (BMB) wet mount should be prepared each time amoebic trophozoites are seen in a saline wet mount, or when their presence is suspected. 18-01-2018 Dr.T.V.Rao MD
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Direct saline and iodine mounts
1. With a wax pencil writes the patient’s name or number and the date at the left-hand end of the slide.
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Preparing a faecal specimen
• Place a drop of saline in the centre of the left half of the slide and place a drop of iodine solution in the centre of the right half of the slide.
• Note: If the presence of amoebic trophozoites is suspected, warm saline (37c) should be used.
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Preparation of Wet film
• With an applicator stick (match or tooth pick), pick up a small portion of the specimen (size of a match head) and mix the drop of saline.
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MACROSCOPIC EXAMINATION
COLOUR
Pale
CONSISTENCY
-Liquid (Troph)-Formed (Cyst)-Semi formed (Cyst)
COMPOSITION
?? Blood ?? Mucus(dysentry)
Adult PARASITES
*Ascaris worm*E. vermicularis*T. saginata
STOOL EXAMINATION
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DIAGNOSIS
DIRECT
UrineStool
SputumBiopsyBlood
Aspirates
INDIRECT
IHATLATIFAT
ELISA
MOLECULAR
PCRDNA probes
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URINE EXAMINATION
MACROSCOPIC
colour
white
Chyluria
Filaria
smoky
Blood
S. haematobium
MICROSCOPIC
Sedimentation
concentration
Membrane filtration
Acetic acid
RBC haemolysis
Clear ova
Ether
Dissolve fat
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Examination1. Put the slide with the mounts on the
microscope stage and focus on the mount with the x10 or low-power objective.
2. Regulate the light in the microscope field with the sub stage diaphragm. You should be able to see objects in the field distinctly. Too much or too little light is not good.
3. Examine the entire coverslip area with the x10 objective; focus the objective on the top left-hand corner and move the slide systematically backwards and forwards, or up and down.
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Examination Cont.
4. When organisms or suspicious material are seen, switch to the high-dry objective, and increase the light by opening the sub stage diaphragm to observe the detailed morphology.
-This is a systematic examination. If mounts are examined in this way, any parasites present will usually be found. If the mount is not examined systematically, parasites may be missed. Examine each microscope field carefully, focusing up and down, before moving to the next field.
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STOOL EXAMINATIONA Rapid Methods
Saline smear Iodine smear
saline Iodine 1%
Huge number of:
•Eggs
• Protozoal troph. Motility
(Amoeb, flagellates)
Huge number of:
•Cyst morphological details
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Need for Concentration Methods for Faecal examination
• A concentration procedure is performed mainly to separate the parasites from faecal debris. The concentration procedure not only increases the numbers of parasites in the sediment but it also unmasks them, making them more visible by removing organic and inorganic debris
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STOOL EXAMINATIONScanty infection
Concentration techniques
Sedimentation Floatation
• Heavy eggs (Ascaris egg)
• Operculated eggs (Trematodes)
• Larvae (Strong sterc.)
• Cysts
• Non Operculated eggs
Trematodes ( S. m.)
CestodeNematode(Hookworms,Trichostong)
• Cysts
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STOOL EXAMINATIONSaline sedimentation
10 g stool
Saline
Mesh wire gauze
Conical flask
Sediment
Emulsify
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STOOL EXAMINATION Kato technique
Mesh screen
Template
Hole
Remove the template
Cellophane soaked by glycerin (clears faeces(
Egg count/ g stool
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Stool examination other Texhniques
• Stoll’s technique for eggs of Ascaris, T. trichiura., Hookworms, S. mansoni
• Baermann’s technique Detec. Of Nematode L. /stool, soil
• Cultures for Nematode larvae using Filter paper culture for Larvae of: St. stercoralis (A,L) and Hookworms
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Artifacts
• Artifacts other things, living or artificial, present in the stool that are not parasites and could mislead the laboratory worker.
• Note: “Artifacts not to be mistaken for cysts”.
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Plant cells
Air bubble
Plant hairsPlant fibre
Pollen grains
Non-human
coccidial oocysts Fat droplets
Soapy plaques
Starch cell Charcot leyden crystals Muscle fibers
Fatty acids Macrophage
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•Round worm•Hook worm•Tape worm•Pin worm•Whipworm
PA R A S I T E
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M I C R O S C O P I C E X A M I N AT I O N
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P I N W O R M E G G C O L L E C T I O N
Eggs of Pin worm – Enterobius vermicularis rarely appear in stools. These are usually collected in the folds of skin in perianal region.
COLLECTION
Cotton swab / Plaster patch – Anus especially in early morning – Dipped in Saline – Observed.
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E X A M I N AT I O N O F PA R A S I T E S
Warm stools are best for detecting Ova orparasites. Do not refrigerate the specimen.
Because of cyclic life cycle of parasites, three separate random stool specimens are recommended for examination.
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N O R M A L VA LU E S
• Undigested food materials – None to small amount
• Starch – None
• Eggs, Cysts, Parasitic fragments – None
• Yeasts – None
• Leukocytes – None
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H O O K W O R M
Ancylostoma duodenale.
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TA P E W O R M
Taenia solium-PorkTaenia saginata-Beef
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W H I P W O R M
Trichuris trichura
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P I N W O R M
Enterobius vermicularis
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E N TA M O E B A
Entamoeba histolytica
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G I A D I A S I S
Giardia lamblia
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Examining other Specimens
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SPUTUM EXAMINATION
MACROSCOPIC
Appearance
Bloody (Parag)
Rusty brown (Parag)
MICROSCOPIC
Concentration
NaOH
Sputum
Centrifuge
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BIOPSY SPECIMEN
SKIN
O. Volvulus mf
MUSCLE BIOPSY
T. Spiralis larvae
RECTAL BIOPSY
Schistosomes egg
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ASPIRATES EXAMINATION
CSF
• Afr. Tryp. (trypom)• FLA (troph)• M.f. of loa loa• L. of T spiralis
Duodenal aspirates
• G. lamb troph• Crypto oocyst• St sterc. Rh L.• Fasciola eggs
BM aspirates
• L. donovani a,ast.•T. cruzi amast.•P. falciparum.
Cutanoeus ucler
•Leishmaniasis
Direct stain (amast)
NNN (promast)
•Lumbar puncutre• Centrifuge•Examine sed.
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BLOOD EXAMINATION
Blood films
Thin Thick
Buffy coat films
QBC techniqueKnott’s conc.
tech.
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BLOOD EXAMINATIONBLOOD FILMS
• Thin • ThickBld drop
spread
Air dry
methyl alcohol
Geimsa
Air dry
Geimsa
Circular motion
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Observe the Thin and Thick Smear
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QBC Method is used in ….
• The QBC Malaria method is the simplest and most sensitive method for diagnosing the following diseases.
• Malaria
• Babesiosis
• Trypanosomiasis (Chagas disease, Sleeping Sickness)
• Filariasis (Elephantiasis, Loa-Loa)
• Relapsing Fever (Borreliosis)
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QBC A QUICKER ALTERNATIVE IN MALARIA
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How to read the QBC results ….
• When the operator looks through the wall of the tube, the nucleus of the parasite fluoresces bright green, and the cytoplasm shows up as yellow-orange. The shape and colours are quite characteristic, and since the parasites are concentrated up to 1000X, there are usually a large number of them in any field of view in this area of the tube.
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URINE EXAMINATIONSEDIMENTATION CONCENTRATION
15-20 min Centrifuge (2 min)
Clean conical glass receptacle
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URINE EXAMINATIONMembrane filtration technique
air
10 ml urine
Nucleopore filter
Eggs of Schistosoma
+ Saline
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URINE EXAMINATION
HELMINTHES
• S. haem.egg• E. vermic. egg• S. mansoni egg• Mf (Ov, Wb)• H sand
PROTOZOA
• T. Vag troph
ARTHROPODES
• Pthirus pubis
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Indirect immunological diagnosis
• Serology – All tests available– IHA
– ELISA
• More useful in– Amoebiasis
– Leishmaniasis
– Malaria
– Toxoplasmosis
– Trichinosis
– Filariasis
– Echinococcosis
• Skin Tests –Specificity low, cross reactions common
–Casoni’s test
–Leishmanin test
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• Program created by Dr.T.V.Rao MD for Basic Learning methods to
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