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Laboratory Diagnosis of
Toxoplasmosis
Outline
Disease Burden of Toxoplasmosis in
India
 The Test Formats available




Antibody Detection
 Detection of Toxoplasma- Microscopy, Animal, Culture
 Detection of Parasite DNA



Application in Clinical Situations



Screening in Pregnancy
Diagnosis in the Neonatal, pre natal stage
Diagnosis in immunocompromised host- Cerebral
Toxoplasmosis




The Disease Burden


In India, the national seroprevalence
has been found to be 24.3%.(Dhumne et
al,2007. J Parasitol;93)





Lowest in the northern parts of India,
and highest in the south.
A high seroprevalence of 57% has been
reported from Almora district (Singh and
Nautiyal 1991. IJMR;93)



A recent study from Chandigarh: 15.33%
pregnant women were
seropositive.(Khurana et al 2010. IJMM;28).
The Disease Burden
Study from Hyderabad showed a
seropositivity (IgG) rate of 27% in
women with BOH, and IgM in 11.5%.
 Study from our centre revealed 9.3%
IgM positivity rate in BOH cases.

The Test Formats:1. Antibody


Remains the test method of choice.

1.

Use of Particulate Antigens:
Trophozoites, IgG





2.




Dye Test
IFAT
Agglutination, Differential Agglutination.

Use of Soluble Antigens: Cytosol
antigen.
ELISA
Avidity Test
Western Blot
1. Antibody Detection
a.







Sabin Feldman Dye Test : IgG
Described in 1948 (Science, 1948:108)
Cytotoxic effect of antibodies in the
presence of complements.
End point is the dilution at which 50%
of the tachyzoites are dead.
Live tachyzoites necessary
Easy to read, Highly sensitive (2 IU/ml)
Detects very early antibodies.
1. Antibody Detection
b. IFAT:
 Formalin treated tachyzoites used
 Can detect IgG, IgM
 Difficult to interpret
 BFP in autoimmune diseases.
1. Antibody Detection
c. Agglutination Test: IgG
 Formalin treated antigen
 Highly sensitive if 2ME treatment is
done.
Differential Agglutination Test :
 Formalin treated antigen(HS) and
methanol treated antigen (AC) used
with a single sample
 To rule out recent infection.
1. Antibody Detection
 AC

antigen specific for membrane,
strong antibody response in early
infection, wanes after 6-12 mts.
 Sensitivity: HS: 2 IU/ml, AC: 50IU/ml
 HS/AC≥ 4 : Infection has occurred
more than 6 months before.
 Antigens difficult to prepare, not
available commercially.
1. Antibody Detection
Use of Soluble antigen: Cytosol
antigens enriched with membrane
antigen( P30, SAG 1) to enhance
sensitivity.
a. ELISA
 Extensively used
 IgG, IgM, IgA, IgE.
 IgG indirect ELISA: Sensitivity 10300 IU/ml.
1. Antibody Detection
b. IgG Avidity Test
 Increasing humoral response, ↑avidity of IgG
 Early stage of infection: Weak avidity; late
stage: Strong avidity
 Two parallel ELISA: Untreated serum; serum
treated with urea/guanidine/thiocyanate
(Dissociates Ag-Ab complex of weak avidity)
 High avidity index→ Infection in remote past
 Caveat: Not always true, ↑in avidity may be
slow
1. Antibody Detection
c. Western Blot Test
 Two samples tested in parallel:
Blood/CSF; Blood/aqueous humor;
Maternal/neonatal blood.
 Additional bands in the second
sample denotes organ/neonatal
infection
IgG and IgM Western blots of
serum from a mother (m)
and her newborn (b). Sera
were drawn from mother and
baby when the baby was 2
days of age.
Toxoplasmawas isolated from
the placental tissue.

Remington et al 2004.
JCM:42.
2. Detection of Toxoplasma
a.



Microscopy:
Smears stained by Giemsa, FAT,
Biopsy material
Presence of foci of tacyzoites with or
without cysts suggest active disease.
2. Detection of Toxoplasma
b. Animal Inoculation
 Body fluids, trypsinized tissue
 Intraperitoneal inoculation in 6-8 mice
 Seroconversion occurs after 7-10
days
 Peritoneal lavage examination shows
the tachyzoites.
2. Detection of Toxoplasma
c. Cell Culture:
 Human embryo fibroblast (MRC5) or
monocyte lines (THP 1).
 4-5 days.
3. PCR


Diagnosis of congenital, ocular, cerebral
toxoplasmosis.
 The most common use of PCR is for
prenatal diagnosis of the congenital
infection using amniotic fluid.
 Most laboratories use the 35-foldrepeated B1 gene
 Some laboratories in Europe are
switching to the AF146527 sequence, a
DNA fragment that is repeated 200- to
300-fold in the T. gondii genome.
3. PCR
An evaluation of three targets (18S
ribosomal DNA, B1, and AF146527) in
parallel.
 Differences in the sensitivity and
specificity of these three PCR
techniques were not found to be
statistically significant ( Filisetti et al 2003.


JCM;41).
Diagnosis in Pregnancy
Active infection normally occur once
in life.
 Acquired immunity is life long
 The risk is only from an infection
caught for the first time during
pregnancy, or 2-3 months before
conception.
 Mothers who tested positive before
the pregnancy do not need
monitoring/screening.

Diagnosis in Pregnancy


Within 2–3 months before conception
- 1% or below risk of transmission but
a high risk of miscarriage

• Severity varies with age of fetus

• More severe manifestation early in
pregnancy, Less frequent transmission
• More frequent transmission later in
pregnancy, Less severe manifestation
Risk of Toxoplasma gondii congenital infection (transmission) and development of clinical
signs in offspring before age 3 years, according to gestational age at maternal
seroconversion.

Goldstein E J C et al. Clin Infect Dis. 2008;47:554-566
© 2008 by the Infectious Diseases Society of America
Diagnosis in Pregnancy
In most centres one sample is tested
for IgG and/or IgM
IgM



◦ Determine recent infection or in the distant past.
◦ Significant potential of misinterpretation of +ve
result, should be confirmed by other tests.
◦ IgM antibodies can persist for months to more
than one year.
◦ Persistence of these IgM antibodies does not
appear to have any clinical relevance .
Interpretation of results of serological tests for toxoplasmosis performed at clinical
(nonreference) laboratories.

Goldstein E J C et al. Clin Infect Dis. 2008;47:554-566
© 2008 by the Infectious Diseases Society of America
Neonatal/Prenatal Diagnosis
Diagnosis in neonatal period : WBT
with paired sample
 IgM and IgA detection may be used:
Chance of false negative because of
small amounts produced.
 Declining IgG level may be used to
rule out congenital infection.
 PCR of amniotic fluid+
Ultrasonogram done after 18 weeks.

Diagnosis in
Immunocompromised Patients
Peripheral blood, BAL, Bone marrow
may be used to demonstrate and/or
isolate the parasite.
 PCR with the above samples.
 If IgG in blood is positive, risk is high
in HIV positive patients with CD4+
count<200/cumm, and IgG >150IU/ml
OR presence of 22,25, or 69KD bands
in WBT.

Conclusion
Disease burden is high in India as
shown by seroprevalence studies.
 There is no regulation for antenatal
screening
 The rural population is highly
vulnerable but totally neglected
regarding testing for this important
pathogen .
 Toxoplasmosis remains a neglected
disease in India.

Laboratory diagnosis of toxoplasmosis

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Laboratory diagnosis of toxoplasmosis

  • 2. Outline Disease Burden of Toxoplasmosis in India  The Test Formats available   Antibody Detection  Detection of Toxoplasma- Microscopy, Animal, Culture  Detection of Parasite DNA  Application in Clinical Situations  Screening in Pregnancy Diagnosis in the Neonatal, pre natal stage Diagnosis in immunocompromised host- Cerebral Toxoplasmosis  
  • 3. The Disease Burden  In India, the national seroprevalence has been found to be 24.3%.(Dhumne et al,2007. J Parasitol;93)   Lowest in the northern parts of India, and highest in the south. A high seroprevalence of 57% has been reported from Almora district (Singh and Nautiyal 1991. IJMR;93)  A recent study from Chandigarh: 15.33% pregnant women were seropositive.(Khurana et al 2010. IJMM;28).
  • 4. The Disease Burden Study from Hyderabad showed a seropositivity (IgG) rate of 27% in women with BOH, and IgM in 11.5%.  Study from our centre revealed 9.3% IgM positivity rate in BOH cases. 
  • 5. The Test Formats:1. Antibody  Remains the test method of choice. 1. Use of Particulate Antigens: Trophozoites, IgG    2.    Dye Test IFAT Agglutination, Differential Agglutination. Use of Soluble Antigens: Cytosol antigen. ELISA Avidity Test Western Blot
  • 6. 1. Antibody Detection a.       Sabin Feldman Dye Test : IgG Described in 1948 (Science, 1948:108) Cytotoxic effect of antibodies in the presence of complements. End point is the dilution at which 50% of the tachyzoites are dead. Live tachyzoites necessary Easy to read, Highly sensitive (2 IU/ml) Detects very early antibodies.
  • 7. 1. Antibody Detection b. IFAT:  Formalin treated tachyzoites used  Can detect IgG, IgM  Difficult to interpret  BFP in autoimmune diseases.
  • 8. 1. Antibody Detection c. Agglutination Test: IgG  Formalin treated antigen  Highly sensitive if 2ME treatment is done. Differential Agglutination Test :  Formalin treated antigen(HS) and methanol treated antigen (AC) used with a single sample  To rule out recent infection.
  • 9. 1. Antibody Detection  AC antigen specific for membrane, strong antibody response in early infection, wanes after 6-12 mts.  Sensitivity: HS: 2 IU/ml, AC: 50IU/ml  HS/AC≥ 4 : Infection has occurred more than 6 months before.  Antigens difficult to prepare, not available commercially.
  • 10. 1. Antibody Detection Use of Soluble antigen: Cytosol antigens enriched with membrane antigen( P30, SAG 1) to enhance sensitivity. a. ELISA  Extensively used  IgG, IgM, IgA, IgE.  IgG indirect ELISA: Sensitivity 10300 IU/ml.
  • 11. 1. Antibody Detection b. IgG Avidity Test  Increasing humoral response, ↑avidity of IgG  Early stage of infection: Weak avidity; late stage: Strong avidity  Two parallel ELISA: Untreated serum; serum treated with urea/guanidine/thiocyanate (Dissociates Ag-Ab complex of weak avidity)  High avidity index→ Infection in remote past  Caveat: Not always true, ↑in avidity may be slow
  • 12. 1. Antibody Detection c. Western Blot Test  Two samples tested in parallel: Blood/CSF; Blood/aqueous humor; Maternal/neonatal blood.  Additional bands in the second sample denotes organ/neonatal infection
  • 13. IgG and IgM Western blots of serum from a mother (m) and her newborn (b). Sera were drawn from mother and baby when the baby was 2 days of age. Toxoplasmawas isolated from the placental tissue. Remington et al 2004. JCM:42.
  • 14. 2. Detection of Toxoplasma a.   Microscopy: Smears stained by Giemsa, FAT, Biopsy material Presence of foci of tacyzoites with or without cysts suggest active disease.
  • 15. 2. Detection of Toxoplasma b. Animal Inoculation  Body fluids, trypsinized tissue  Intraperitoneal inoculation in 6-8 mice  Seroconversion occurs after 7-10 days  Peritoneal lavage examination shows the tachyzoites.
  • 16. 2. Detection of Toxoplasma c. Cell Culture:  Human embryo fibroblast (MRC5) or monocyte lines (THP 1).  4-5 days.
  • 17. 3. PCR  Diagnosis of congenital, ocular, cerebral toxoplasmosis.  The most common use of PCR is for prenatal diagnosis of the congenital infection using amniotic fluid.  Most laboratories use the 35-foldrepeated B1 gene  Some laboratories in Europe are switching to the AF146527 sequence, a DNA fragment that is repeated 200- to 300-fold in the T. gondii genome.
  • 18. 3. PCR An evaluation of three targets (18S ribosomal DNA, B1, and AF146527) in parallel.  Differences in the sensitivity and specificity of these three PCR techniques were not found to be statistically significant ( Filisetti et al 2003.  JCM;41).
  • 19. Diagnosis in Pregnancy Active infection normally occur once in life.  Acquired immunity is life long  The risk is only from an infection caught for the first time during pregnancy, or 2-3 months before conception.  Mothers who tested positive before the pregnancy do not need monitoring/screening. 
  • 20. Diagnosis in Pregnancy  Within 2–3 months before conception - 1% or below risk of transmission but a high risk of miscarriage • Severity varies with age of fetus • More severe manifestation early in pregnancy, Less frequent transmission • More frequent transmission later in pregnancy, Less severe manifestation
  • 21. Risk of Toxoplasma gondii congenital infection (transmission) and development of clinical signs in offspring before age 3 years, according to gestational age at maternal seroconversion. Goldstein E J C et al. Clin Infect Dis. 2008;47:554-566 © 2008 by the Infectious Diseases Society of America
  • 22. Diagnosis in Pregnancy In most centres one sample is tested for IgG and/or IgM IgM  ◦ Determine recent infection or in the distant past. ◦ Significant potential of misinterpretation of +ve result, should be confirmed by other tests. ◦ IgM antibodies can persist for months to more than one year. ◦ Persistence of these IgM antibodies does not appear to have any clinical relevance .
  • 23. Interpretation of results of serological tests for toxoplasmosis performed at clinical (nonreference) laboratories. Goldstein E J C et al. Clin Infect Dis. 2008;47:554-566 © 2008 by the Infectious Diseases Society of America
  • 24. Neonatal/Prenatal Diagnosis Diagnosis in neonatal period : WBT with paired sample  IgM and IgA detection may be used: Chance of false negative because of small amounts produced.  Declining IgG level may be used to rule out congenital infection.  PCR of amniotic fluid+ Ultrasonogram done after 18 weeks. 
  • 25. Diagnosis in Immunocompromised Patients Peripheral blood, BAL, Bone marrow may be used to demonstrate and/or isolate the parasite.  PCR with the above samples.  If IgG in blood is positive, risk is high in HIV positive patients with CD4+ count<200/cumm, and IgG >150IU/ml OR presence of 22,25, or 69KD bands in WBT. 
  • 26. Conclusion Disease burden is high in India as shown by seroprevalence studies.  There is no regulation for antenatal screening  The rural population is highly vulnerable but totally neglected regarding testing for this important pathogen .  Toxoplasmosis remains a neglected disease in India. 