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Thick film interpretation: Difference between revisions

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<span style="font-size:90%">Some strengths and weaknesses of each approach are summarised in the table below:</br></span>
<span style="font-size:90%">Some strengths and weaknesses of each approach are summarised in the table below:</br></span>


<div style="width: 95%; font-size:90%;">
{| class="wikitable" style="border-style: solid; border-width: 4px; color:black"
!colspan="3" style = "background:#e1f1fd; border:solid; border-width: 3px;"|<span style="font-size:90%;">'''COMPARISON OF THICK AND THIN FILMS'''</span></br>
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! Feature !! Thick Film !! Thin Film
|-
| Sensitivity for detection || Higher: detects low parasitaemia ~5–10 parasites/µL || Lower: generally needs ~50 parasites/µL for reliable detection)
|-
| Species Identification || Poor: RBC morphology lost and species-specific features may be difficult || Excellent: Parasite morphology and RBC characteristics are readily observed
|-
| Quantification of parasitaemia || Difficult: requires estimation so is imprecise || Easier: parasites can be counted per number of RBCs
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| Preparation and staining || Longer: requires air drying before careful staining to avoid artefact || Faster: films are fixed and stained immediately with clearer morphology
|}
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Revision as of 11:07, 13 February 2025


OVERVIEW OF THICK FILMS


A thick film is prepared by placing a small drop of blood on a slide then spreading it in a circular motion. The thick layer acheived is then air-dried without fixation.
IMAGE
The principles are:

  • The blood layer will be many layers thick (varying from 6-20 accross the specimen)
  • The erythrocytes are unfixed, so will be lysed during staining appearing only as debris.
  • The Giemsa stain will stain and distinguish the remaining white cells and parasites.
  • This concentration effect allows parasites to be detected with high sensitivity


Typical appearances of a case of P.falciparum with easily detected trophozoites are shown below.

  • Low magnification view for scale, 3 regions marked

    Low magnification view for scale, 3 regions marked

  • Region A: a single disrupted trophozoite

    Region A: a single disrupted trophozoite

  • Region B: 5 trophozoites in three group

    Region B: 5 trophozoites in three group

  • Region C: 2 trophozoites in one group

    Region C: 2 trophozoites in one group

"


Note the differences in recognition - the typical ring form and vacuole of the parasite are not as easy to distinguish and chromatin dots may appear to separate from parasite cytoplasm while the absence of intact red cells takes away important clues to parasite size, distribution within the red cell, and any red cell changes. This is illustrated in the image below

  • Two ring frms of P.falciparum

    Two ring frms of P.falciparum

  • High-power image of the parasites

    High-power image of the parasites


Detailed Sections:

1. Click for a comparison of thick and thin films

COMPARISON THICK vs THIN
DISTINGUISHING PARASITES vs DEBRIS
DISTINGUISHING SPECIES
IDENTIFYING PIGMENT
Some strengths and weaknesses of each approach are summarised in the table below:

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