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Cryptosporidium parvum

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Title: Cryptosporidium parvum

1
Cryptosporidium parvum
Small in size 5x4.5 µm C. Parvum oocyst
2
Cryptosporidium parvum

Enteric parasite
One of the three most common diarrhea-causing
pathogens in the world

3
Prevalence

Found in most parts of the world
Most prevalent in Asia, Africa, Australia, South
America
Antibody prevalence in Peru and Venezuela 64
32 in Peace Corps workers
More prevalent in rural areas of U.S.

4
Transmission

Fecal-oral route
Fomites
Water
Drinking water (even after treatment)
Swimming pools
Unpasteurized Apple Cider
Animal contact
Food

5
Infectivity

Can be infected by just one oocyst
10 billion oocysts per gram infected feces

6
Life Cycle
7
Life Cycle
Life cycle
8
Oocyst

Double walled
Resistant to chlorine, drying, progressive
freezing, salt water
Only stage in life cycle that can live ex vivo
Imbeds itself in gut epithelium and releases
sporozoites
Reproduction continues sexually and asexually

9
Clinical Characteristics

Secretory diarrhea (some mucous, but no blood)
Slight fever, fatigue, myalgia
Oocysts may infect the lungs and trachea,
resulting in cough
Dehydration and extreme weight loss in
immunocompromised

10
Laboratory diagnosis of cryptosporidiosis
Cryptosporidium spp.

Basic guidelines
A. Multiple stool specimens (at least 3) should
be tested before a negative result is reported.
B. To maximize recovery of oocysts, stool
specimens in formalin, or other fixatives, should
be concentrated prior to microscopic examination
(e.g.,10 min at 500 g when using the formalin

ethyl-acetate concentration procedure).
Exception Specimens to be used for rapid
car-tridge assays should NOT be concentrated
because antigens are lost during the procedure!
C. Choice of diagnostic techniques depends on
available equipment and reagents, experience,
and considerations of time and cost.

12
1. Wet mount

In bright-field microscopy using differential
interference contrast (DIC), oocysts appear as
small round structures (4 to 6 µm) similar to
yeasts. They do not auto fluoresce.

13
2. Modified acid-fast stain

Oocysts (4 to 6 µm) often have distinct oocyst
walls and stain from light pink to bright red.
However, staining may be variable. In particular,
infections that are resolving can have colorless
oocyst ghosts. Mature oocysts may have
discernible sporozoites (up to 4).

Modified acid-fast oocyst stain
14
3. Direct fluorescent antibody (DFA) assay

This technique offers the highest combination of
sensitivity and specificity and is considered the
gold standard by many laboratories. However, it
does not provide a stained slide that can be
archived. It requires special equipment
(fluorescence microscope) and commercially
available test kits.

15
Sensitivity and specificity

Sensitivity and specificity are statistical
measures of the performance of a binary
classification test. The sensitivity (also called
recall rate in some fields) measures the
proportion of actual positives which are
correctly identified as such (i.e. the percentage
of sick people who are identified as having the
condition) and the specificity measures the
proportion of negatives which are correctly
identified (i.e. the percentage of well people
who are identified as not having the condition.

16
Definitions Imagine a scenario where people are
tested for a disease. The test outcome can be
positive (sick) or negative (healthy), while the
actual health status of the persons may be
different. In that setting -True positive Sick
people correctly diagnosed as sick -False
positive Healthy people wrongly identified as
sick -True negative Healthy people correctly
identified as healthy -False negative Sick
people wrongly identified as healthy
17
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18
Other methods for detecting Cryptosporidium in
stool.
6. Enzyme immunoassay (EIA) The EIA does not
rely on microscopy skills, is highly sensitive
and specific, and is useful for screening large
numbers of specimens.
19
Cell-free culture ofCryptosporidium parvum

Simple technique for culturing Cryptosporidium
without host cell interference.
The potential of improving routine water and
other environmental monitoring for
Cryptosporidium.
Contribute much to our understanding of the
developmental and evolutionary biology of
Cryptosporidium.

20
Amplification of oocysts

In Vivo
- Large animal Lambs
- Small animal Neonatal mice
In Vitro
- Cell cuture

21
In Vitro Cultivation

Oocysts preparation
- neonatal mice
- Inoculation with 100,000-120,000 oocysts per
mouse by gastic tube
After 7 day post infection, mice will be
killed and collected intestinal part.
Extraction and purification

22
In Vitro Cultivation

Media preparation
Excystation media
Sterile Acidic water (pH2.5-3.0) Trypsin
EDTA(0.5) 45 µl

Cell free cultivation
Put 350,000 oocysts from stock into 9 ml of
excystation media.
Incubate 30 min at 37 C with shaking every 5
min.
spin down at 3,500 rpm 10 min
Aspirate excystation media
Resuspend pellet with 10 ml of maintenance media
and mix well
Add 10 ml of maintenance media into 25cm2 flask
Add 5 ml of oocysts in maintenance media into the
flask
Leaving amount of Cryptosporidium oocysts
maintenance
for checking excystation rate
Incubate at 37 C with 5 CO2

24
24 hrs after culture
trophozoite
empty shell
Sporozoite
25
48-72 hrs after culture
Meront type 1
26
48-72 hrs after culture
Meront type II
27
6 day after culture
Macrogamete and Microgamete
28
7-8 after culture