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Medical Parasitology Lab. Medical Parasitology Lab.

Medical Parasitology Lab. - PowerPoint Presentation

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Medical Parasitology Lab. - PPT Presentation

Introduction Topics Introduction Sample Collection and Preservation Methods Wet mount Preparation Normal saline 085 Iodine BMB Artifacts Concentration Techniques Modified Formal Ether Sedimentation technique ID: 277266

medical lab 2012 parasitology lab medical parasitology 2012 raed ahmed stool examination specimen fecal preserved mount parasites samples wet

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Slide1

Medical Parasitology Lab.

Introduction Slide2

Topics

Introduction

Sample Collection and Preservation Methods Wet mount PreparationNormal saline 0.85%IodineBMB Artifacts Concentration TechniquesModified Formal- Ether Sedimentation techniqueAcid- Ether Sedimentation techniqueFlotation TechniquesBy using Sheather’s solutionBy using Sodium Chloride solution Staining of parasites

Raed Z. Ahmed, Medical Parasitology Lab.,2012Slide3

Detecting of Blood ParasitesThick and thin Blood smearCounting of Helminthes Eggs in Feces

Chemical Tests

Fecal PH test

Testing feces for Occult BloodFecal fat testStool reducing sugar testMedical EntomologyTopics (cont.) Raed Z. Ahmed, Medical Parasitology Lab.,2012Slide4

Quizzes: ــــــــــــــــــــــــــــــــــــــــــــــــــــــــــــــ10%Assignment & Participation: ــــــــــــــــــــــــ

10%

Midterm examination:

ــــــــــــــــــــــــــــــــــــ 30%Final examination: ــــــــــــــــــــــــــــــــــــــــــ50%Practical exam: ـــــــــــــــــــــــــــــــــــ20%Written exam: ـــــــــــــــــــــــــــــــــــــ30%Grades Raed Z. Ahmed, Medical Parasitology Lab.,2012Slide5

General Lab Objectives To familiarizes the student with the most widely used techniques for detection of parasites.

To be able to identify the parasite stages.

To learn the student, how to deal with risk samples.

Raed Z. Ahmed, Medical Parasitology Lab.,2012Slide6

What is the stool or feces?Waste residue of indigestible material (cellulose during the previous 4 days),

Bile pigments and

electrolyte,

Intestinal secretions, including mucus,Leukocytes that migrate from the bloodstream,Epithelial cells that have been shade,Bacteria and Inorganic material(10-20%) chiefly calcium and phosphates. Undigested and unabsorbed foodRaed Z. Ahmed, Medical Parasitology Lab.,2012Slide7

Fecal Specimen

Fecal specimen are examined for protozoa, helminthes larvae or eggs.

The stages of protozoa found in stool samples are trophozoites and cysts or oocysts.

The stages of helminthes usually found in the stool samples are eggs and larvae, through whole adult worms or segment of worms may also be seen.Adult worms and segment of tape worms are usually visible to naked eye, but eggs, larvae, cyst, oocyst and trophozoites can be seen only with the microscope.In order to see these structure, the fecal material must be properly collected and examined.Raed Z. Ahmed, Medical Parasitology Lab.,2012Slide8

Parasites stagesSlide9

Number of Specimens and Collection TimeNo technique is 100% successful in detecting parasites by 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 free in the faeces.

Because of the intermittent passage of certain parasites, the possibility of finding organisms is increased by examining multiple specimens.

It is suggested that 3 specimens, collected at 2 to 3 day intervals, should be examined both pretreatment and post treatment (to ensure eradication of documented pathogenic protozoa).

Raed Z. Ahmed, Medical Parasitology Lab.,2012Slide10

Collection of Fecal Specimen

Because of fragile nature of many intestinal parasites, and the need to maintain their morphology for accurate identification.

Reliable microscopic diagnosis can not made unless the stool is collected properly.

The stool specimen must be enough for satisfactory examination of fresh feces uncontaminated by urine, dirt*, water or other body secretion such as menstrual blood. If the sample is too small or contaminated with urine, it should not be accepted. Ask the patient to pass another specimen. Raed Z. Ahmed, Medical Parasitology Lab.,2012Slide11

Raed Z. Ahmed, Medical Parasitology Lab.,2012Collection of Fecal Specimen

(cont.)

Collect the specimen in a clean dry screw-capped top container

Collect the stool with a clean tongue blade or similar object.The container should be free from antiseptics and disinfectant. Random specimen: suitable for qualitative testing for blood and microscopic examination.Timed specimen: for quantitative fecal testing such as fecal fat testing, because of the variability of bowel habit and the transit time required for food to pass through the digestive tract, so the most representative sample is a-3 day collection. Slide12

Raed Z. Ahmed, Medical Parasitology Lab.,2012The container with the specimen should be clearly labeled with the following:Patient’s name or number.

Date and time of collection.

All samples should be accompanied by a requisition form from the physician giving relevant clinical details and recent travel

history. Samples and forms from patient with a confirmed or suspected diagnosis of certain infectious diseases such as AIDS or hepatitis should be clearly labeled with “Biohazard”Collection of Fecal Specimen (cont.)Slide13

Raed Z. Ahmed, Medical Parasitology Lab.,2012Most 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 faeces specimen to retain

morphology.

Formed samples can be kept in a refrigerator at 4 C° for a short time, but not in incubator.

Any whole worms or segments passed should be placed in a separate containerCollection of Fecal Specimen (cont.)Slide14

Raed Z. Ahmed, Medical Parasitology Lab.,2012Preservation methods for fecal specimens

Preservation allows

fecal

samples to be examined after a delay in delivery or postage or testing.Many methods for the preservation of stool samples and permanent staining procedures.The most common fixatives are: Polyvinyl Alcohol, PVA Merthiolate Iodine Formalin, MIF Sodium acetate Acetic acid Formalin, SAF Formalin. Bayer’s solution*

The preservatives used have different effect on the various stages of the parasites. Slide15

Raed Z. Ahmed, Medical Parasitology Lab.,2012

Formalin

Formalin 4% has been used for many years as an all purpose fixative that is appropriate for helminthes eggs and larvae and for protozoan cyst.

The fixative has a long shelf life.Concentration methods, like formalin- ether concentration can be performed from the preserved stool samples without loss of concentration abilities.The major disadvantage of formalin is that permanent staining procedures can't be performed from formalin preserved stool samples. Slide16

Raed Z. Ahmed, Medical Parasitology Lab.,2012

PVA

This fixative is recommended for the preservation of the trophozoite and cyst stages of the intestinal protozoa, and also suitable for helminthes eggs and larvae.The preservation of the two stages of protozoa is excellent.The PVA is a plastic resin that serves as adhesive for the stool material.Has a long shelf life ( months to years ).Concentration methods can’t performed from the specimen preserved by PVA.Slide17

Raed Z. Ahmed, Medical Parasitology Lab.,2012The greatest advantage of this fixative is that a permanent stain can be prepared from stool specimen preserved by PVA, giving excellent result with trichrome staining.

Specimen preserved by PVA can’t be used with immunoassay kits.

Toxic, because contain mercury compound.

PVA (cont.) Slide18

Raed Z. Ahmed, Medical Parasitology Lab.,2012

SAF

Good routine fixative for protozoan cyst and trophozoites, helminthes eggs, and larvae.

Has long shelf life. ( months to years).The preserved stool samples permits concentration techniques, most monoclonal detection kits, and permanent staining.Unlike the PVA, the SAF fixative has poor adhesive properties when SAF preserved samples are used to prepare permanent stained smears. ( Mayer’s albumin has been recommended as an adhesive.The combination of SAF preserved material and CB, IHK, and mod. Ziel Neelsen provides excellent staining of protozoan where staining of SAF preserved material with Trichrome gives poor results.Slide19

Raed Z. Ahmed, Medical Parasitology Lab.,2012

SAF

(cont.)

Specific advantages of the use of SAF are:SAF preserved material can be used for concentration techniques and permentant stained smears (CB, IHK).SAF preserved material can be used for some immunoassay methods.SAF is easy to prepare and has a long shelf life.Unlike the PVA, the SAF fixative contain no mercury compounds. It is therefore much less toxic than PVASlide20

Raed Z. Ahmed, Medical Parasitology Lab.,2012

MIF

This fixative was originally developed as a screening procedure for intestinal parasites.

MIF combines preservation and staining for most kinds and stages found in faeces.It’s contains Merthiolate, Iodine, and Formalin.The preserved material permits concentration techniques.The major disadvantages are the short shelf life ( duo to iodine) and permanent stained smears can’t be prepared from MIF preserved material.Slide21

Raed Z. Ahmed, Medical Parasitology Lab.,2012Fixative used for the preservation of stool samples: an overview of the advantages and disadvantages:

Formalin 4%

PVA

SAFMIFToxicity+/-+++ ( duo to Hg ) +/-+/-Shelf life

Long

(months)

Long

(months/years)

Long

(months/years)

Limited

Preparation

Easy

Difficult

Easy

Easy

Quality of fixation

Egg: ++

Egg: ++

Egg: ++

Egg: ++

Cyst: ++

Cyst: +++

Cyst: ++

Cyst: ++

Troph’s: +/-

Troph’s: +++

Troph’s: +++

Troph’s: ++

Formalin ether concentration

Possible

Not possible

Possible

Possible

Permanent stained

smear

Not possible

Only Trichrome

IHK, CB, mod.

Ziel Neelsen

Not possibleSlide22

Raed Z. Ahmed, Medical Parasitology Lab.,2012Preservation of worms

Cestodes

Wash in water to remove the mucus. Large tapeworms such as

Taenia can be washed for several hours to relax the musculature, and can then be fixed in 10% formol saline b/w two glass slides to give flatter specimens.TrematodesThese should be treated in a similar manner to cestodes, and mounted with the ventral sucker uppermostNematodes Adult are washed in saline to remove mucus. Worms up to about 7 cm in length are fixed in hot(60-70˚C) 70% alcohol, which straightens out living worms, except those which have natural curvatures at the head or the tail. Alternatively, they can be fixed in hot 5% formalin. Large worms such Ascaris lumbricoides can be fixed and preserved in cold 5% formalin Slide23

Stool AnalysisA stool analysis is a series of tests done on a stool (feces) sample to help diagnose certain conditions affecting the

digestive

tract .

These conditions can include infection (such as from parasites, viruses, or bacteria), poor nutrient absorption, or cancer. Raed Z. Ahmed, Medical Parasitology Lab.,2012Slide24

Laboratory analysis includes macroscopic, microscopic examination, chemical tests, and microbiologic tests.The stool will be checked for color, consistency, weight (volume), shape, odor, and the presence of mucus and parasites stages.

The

stool may be examined for hidden (occult) blood, fat, meat fibers, bile, white blood cells, and sugars called reducing substances.

The pH of the stool also may be measured. A stool culture is done to find out if bacteria may be causing an infection.Stool Analysis (cont.)Raed Z. Ahmed, Medical Parasitology Lab.,2012Slide25

Macroscopic ExaminationColorConsistency

abnormal features

adult worm or segment

Microscopic ExaminationWBC/ HPFRBC/ HPF

Mucus

Yeast

Cyst, trophozoite, or both

Larvae, egg, or both

Chemical Examination

Fecal PH test

Fecal fatty acid testing

Testing feces for Occult Blood

Fecal Sample Examination

Stool reducing substances testing

Raed Z. Ahmed, Medical Parasitology Lab.,2012Slide26

Raed Z. Ahmed, Medical Parasitology Lab.,2012Macroscopic Examination

Color:

Brown is normal color, results from the intestinal oxidation of stercobilinogen to urobilin. Bright red to dark red to black stools occur when iron or bismuth is taken or when there is intestinal hemorrhage.Pale yellow stools indicate the biliary obstruction, steatorrea, and also associated with diagnostic procedures that use barium sulfate.White stools occur when there is obstructive jaundice.Green stool may observed in patient taking oral antibiotic, because of oxidation of bilirubin to biliverdin.Slide27

Raed Z. Ahmed, Medical Parasitology Lab.,2012

Consistency:

degree of moisture, will be a guide as to whether the trophozoite stage or the cyst stage of protozoa is likely to present. Formed, write “F” Soft , write “S” Loose , write “L” Watery , write “

W

Macroscopic Examination

(cont.)

Slide28

Raed Z. Ahmed, Medical Parasitology Lab.,2012Macroscopic Examination

(cont.)

Abnormal features:If mucus is present writ “M”, and “B” if blood is present.The presence of mucus coated stool is indicative for intestinal inflammation or irritation. Adult worm or segmentsThe feces may have adult helminthes or segments present such as

Ascaris lumbricoides,

Enterobius

vermicularis

,

or

Taenia

spp.

gravid segment, these can be seen by naked eye.

And frequently motile for several days and may migrate to the top of the container.Slide29

Raed Z. Ahmed, Medical Parasitology Lab.,2012Notice

If several specimens are received at the same time; those containing blood and mucus should be examined first, followed by liquid specimens. These specimens are the most likely to contain amoebic trophozoites ( which die soon after being passed), and must be examined within 1 hour after passage.

Formed specimens may be examined at any time during the first day, but should not be left overnight ( cyst may disintegrate).

Excessive bulky stools may indicate conditions such as giardiasis.Slide30

Raed Z. Ahmed, Medical Parasitology Lab.,2012Microscopic Examination of wet mount

Wet mount is the simplest and easiest technique for the examination of feces, and this method should be performed in all laboratories at peripheral level.

A wet mount can be prepared directly from fecal material or from concentrated specimens.

The basic types of wet mount that should be used for each fecal examination are normal saline (0.85% NaCl), iodine, and buffered methylene blue.Slide31

Raed Z. Ahmed, Medical Parasitology Lab.,2012 The Saline Wet Mount

Is used for the initial microscopic examination of stool specimens.

It is employed primarily to demonstrate worms eggs, larvae. Protozoan trophozoites, and cysts.

This type of mount can also reveal the presence of red blood cells and white blood cells.If the presence of amoebic trophozoites is suspected, warm saline (37˚C) should be used.Microscopic Examination of wet mount (cont.)Slide32

Raed Z. Ahmed, Medical Parasitology Lab.,2012 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.Trophozoite can not be revealed by this type of wet mount, because iodine kill trophozoite.Microscopic Examination of wet mount (cont.)Slide33

Raed Z. Ahmed, Medical Parasitology Lab.,2012Microscopic Examination of wet mount

(cont.)

The

Buffered Methylene Blue Wet MountShould be prepared each time amoebic trophozoites are seen in a saline wet mount, or when their presence is suspected.BMB stains amoebic trophozoites, but not stain amoebic cysts, flagellate trophozoites or flagellate cysts.BMB stain is appropriate only for fresh unpreserved specimens.BMB stain live organism only, it isn’t used on preserved samples in which the organism have been killedWait for five minutes to allow the stain to penetrate the trophozoites. It will overstrain the trophozoites in 30 minutes.Slide34

Notice

Formed stool:

take the portion of stool from an area to include inside and outside parts of the specimen.

Stool with mucus: if mucus is present, label a second slide with the patient’s name or number. Put a drop of saline on the slide, pick up a small portion of mucus and mix with the saline. Trophozoites, if present, are sometimes more readily found in mucus than in the solid parts of the stool.Loose watery stool: if mucus is not present, pick up a small portion of the stool (any part) and mix with the saline.Raed Z. Ahmed, Medical Parasitology Lab.,2012Slide35

Materials and reagents: Microscopic slides.

Cover

slips.

Applicator sticks. Marker or pen for labeling. Reagents: Saline solution(isotonic) Lugols iodine(1% solution)BMBMaking Direct smear MicroscopyRaed Z. Ahmed, Medical Parasitology Lab.,2012Slide36

Wet mount procedures

Examine the slide on microscope:

10X

40XRaed Z. Ahmed, Medical Parasitology Lab.,2012Slide37

Result of ExaminationIf no parasites are found:“No ova or parasites seen

”, and specify whether this result was obtained by direct examination or by a concentration method (name method used).

Never state categorically: “

No parasites”If any parasites are seen, write the scientific name of the parasite with stagesExample: Giardia lambilia cystRaed Z. Ahmed, Medical Parasitology Lab.,2012