Post on 16-Apr-2017
LABORATORY DIAGNOSIS OF MALARIA20 February 2013Shridhan Anand Patil
• Introduction
• Light microscopy
• Antigen detection - Rapid malaria diagnosis tests
(RDTs)
• Serology
• Other
• QBC - PCR
• Summary
Introduction• Accurate diagnosis of malaria
• Chloroquine-resistant malaria
• Ideal test
• Rapid - Easy to use - Reproducible
• Minimum equipment
• Detection of all species
• Quantification of infection
• Response to therapy
• Revert on treatment - Clinical diagnosis
Light microscopy
• Gold standard
• 0.0001% parasitemia detection(5-10/microL)
• Species identification
• Response to therapy
• Thin and thick smears
Interpreting Thick and Thin Films• THICK FILM
• lysed RBCs
• larger volume
• 0.25 μl blood/100 fields
• good screening test
• positive or negative
• parasite density
• more difficult to diagnose
species
• THIN FILM
• fixed RBCs, single layer
• smaller volume
• 0.005 μl blood/100 fields
• good species differentiation
• requires more time to read
• low density infections can be
missed
Recognizing Malaria Parasites
Inside a red blood cell
One or more red chromatin dots
Blue cytoplasm
RING TROPHOZOITE
SCHIZONT GAMETOCYTE
BlueCytoplasm
RedChromatin
BrownPigment
Recognizing Erythrocytic Stages:Schematic Morphology
Malaria Parasite Erythrocytic Stages
Ring form
TrophozoiteSchizont
Gametocytes
Plasmodium falciparum
Rings: double chromatin dots; accole forms;multiple infections in same red cell
Gametocytes: mature (M)andimmature (I) forms (I is rarelyseen in peripheral blood)
Trophozoites: compact(rarely seen in
peripheral blood)
Schizonts: 8-24 merozoites(rarely seen in peripheral blood)
Infected erythrocytes: normal size
M I
Plasmodium vivax
Trophozoites: ameboid; deforms the erythrocyte
Gametocytes: round-oval Schizonts: 12-24 merozoites
Rings
Infected erythrocytes: enlarged up to 2X; deformed; (Schüffner’s dots)
Plasmodium ovaleInfected erythrocytes: moderately enlarged (11/4 X); fimbriated; oval; (Schüffner’s dots)
“malariae - like parasite in vivax - like erythrocyte”
RingsTrophozoites: compact
Schizonts: 6-14 merozoites; dark pigment; (“rosettes”)
Gametocytes: round-oval
Infected erythrocytes: size normal to decreased (3/4X)
Plasmodium malariae
Trophozoite:compact
Trophozoite:typical band form
Schizont:6-12 merozoites;coarse, dark pigment
Gametocyte:round; coarse,dark pigment
Species Differentiation on Thin FilmsFeature P. falciparum P. vivax P. ovale P. malariae
Enlarged infected RBC + +
Infected RBC shape round round, distorted
oval, fimbriated
round
Stippling infected RBC Mauer clefts Schuffner spots
Schuffner spots
none
Trophozoite shape small ring, appliqu
large ring, amoeboid
large ring, compact
small ring, compact
Chromatin dot often double single large single
Mature schizont rare, 12-30 merozoites
12-24 merozoites
4-12 merozoites
6-12 merzoites
Gametocyte crescent shape large, round
large, round
compact, round
Species Differentiation on Thin Films
P. falciparum P. vivax P. ovale P. malariae
Rings
Trophozoites
Schizonts
Gametocytes
Species Differentiation on Thick FilmsFeature P. falciparum P. vivax P. ovale P. malariae
Uniform trophozoites +
Fragmented trophozoites ++ +
Compact trophozoites + +
Pigmented trophozoites +
Irregular cytoplasm + +
Stippling (“RBC ghosts”) + +
Schizonts visible very rarely often often often
Gametocytes visible occasionally usually usually usually
Calculating Parasite Density - 1
• Using 100X oil immersion lens, select area with 10-
20 WBCs/field
• Count the number of asexual parasites and white
blood cells in the same fields on thick smear
• Count ≥ 200 WBCs
• Assume WBC is 8000/l (or count it)
parasites/l = parasites counted WBC counted X WBC count/l
Parasitemia and clinical correlatesParasitemia Parasites /l Remarks
0.0001-0.0004% 5-20 Sensitivity of thick blood film
0.002% 100 Patients may have symptoms below this level, where malaria is seasonal
0.2% 10,000 Level above which immunes show symptoms
2% 100,000 Maximum parasitemia of P.v. and P.o.
Parasitemia and clinical correlatesParasitemia Parasites/l Remarks
2-5% 100,000-250,00
Hyperparasitemia/severe malaria*, increased mortality
10% 500,000 Exchange transfusion may be considered/ high mortality
*WHO criteria for severe malaria are parasitemia > 10,000 /l andsevere anaemia (haemaglobin < 5 g/l).Prognosis is poor if > 20% parasites are pigment containing trophozoites and schizonts (more mature forms) and/or if > 5% of neutrophils contain visible pigment.Hänscheid T. (1999) Diagnosis of malaria: a review of alternatives to conventionalmicroscopy. Clin Lab. Haem. 21, 235-245.
Estimating Parasite DensityAlternate Method
• Count the number of asexual parasites per high-power field (HPF) on a thick blood film
+ 1-10 parasites per 100 HPF++ 11-100 parasites per 100 HPF+++ 1-10 parasites per each HPF++++ > 10 parasites per each HPF
Malaria Antigen Detection• Cannot detect mixed
infections• Cross reactivity with
rheumatoid factor reportedly corrected
Malaria Serology – antibody detection
• Not routinely used for diagnosis
• Transfusion blood screening
• Investigation of cryptic malaria
• Epidemiological purposes
• Blood stage antigen used
Polymerase Chain Reaction
• Specific amplification of malaria DNA
• Excellent sensitivity and specificity
• Detects as low as ≥ 1 parasite/µL of blood
• Useful in identifying drug resistence
• Low parasitemia, therapeutic response
• Species identification – P. knowlesi
Quantitative buffy coat
Summary
• Conventional peripheral smear examination is the gold
standard
• RDTs are costly andrequire quality control
• Serological tests are suitable for epidemiological purpose
• Molecular-biological techniques are suitable for research
labs, quantification, drug resistence detection and species
detection
References• UpToDate – Malaria diagnosis• Lab diagnosis of Malaria. J Clin Pathol 1996;49:533-538• Malaria Diagnosis: A Brief Review. Korean J Parasitol.
Vol. 47, No. 2: 93-102, June 2009 DOI: 10.3347/kjp.2009.47.2.93
• Rapid Diagnostic Tests for Malaria Parasites. CLINICAL MICROBIOLOGY REVIEWS,66–78.2002. Jan. 2002, p. 66–78