| Literature DB >> 35669051 |
Sara M Elzeky1, Nairmen Nabih1, Aida A Abdel-Magied1, Dina S Abdelmagid2, Aya E Handoussa1, Marwa M Hamouda1.
Abstract
Toxoplasma gondii is a parasite with a special predilection for the central nervous system. Toxoplasmosis's contribution to the triggering of many neurodevelopmental disorders was established. This study aimed to detect the seroprevalence and genotypes of T. gondii strains in children with neurodevelopmental disorders. The study included 180 children with neurodevelopmental disorders and 180 children in the control group. Assessment of seropositivity of Toxoplasma IgM and IgG antibodies in patients and controls was carried out. Genetic characterization of T. gondii was obtained by nested polymerase chain reaction (PCR) and restriction fragment length polymorphism (RFLP) technique targeting dense granule gene (GRA6). Our results showed that the overall seroprevalence of T. gondii antibodies in the patient and controls was 35.6% and 11.7%, respectively. Nested PCR showed positivity in 11.1% of the patient group for T. gondii DNA. T. gondii seropositivity rate was significantly high in patients with hydrocephalus and also in patients with epilepsy. Positive nested PCR was significantly high in children with hydrocephalus only. Genotyping using nested PCR-RFLP showed genotype I (80%) followed by atypical strains (20%) with no association with any specific clinical presentation. In conclusion, among toxoplasmosis-positive children with neurodevelopmental disorders, analysis of T. gondii GRA6 locus revealed the predominance of type I genotype followed by atypical strains.Entities:
Year: 2022 PMID: 35669051 PMCID: PMC9166983 DOI: 10.1155/2022/2343679
Source DB: PubMed Journal: J Trop Med ISSN: 1687-9686
Toxoplasmosis seroprevalence and molecular positivity rates among the patient group (children with neurodevelopmental disorders) and control group.
| Parameter | Study participants |
| |
|---|---|---|---|
| Patient group ( | Control group ( | ||
| Overall anti-Toxoplasma antibodies seroprevalence | 64 (35.6) | 21 (11.7) | <0.001 |
| Anti-toxoplasma IgM seropositivity | 18 (10) | 2 (1.1) | 0.04 |
| Anti-toxoplasma IgG seropositivity | 42 (23.3) | 18 (10) | <0.001 |
| Anti-toxoplasma IgM and IgG seropositivity | 4 (2.2) | 1 (0.5) | 0.78 |
| Anti-toxoplasma IgG concentration (IU/ml)∗ | 309.83 (33.9–409.65) | 61.13 (35.76–97.8) | <0.001 |
| Positive PCR for Toxoplasma DNA | 20 (11.1) | 1 (0.5) | 0.03 |
n: number of participants. Data was represented as medium and range (Min–Max).
Figure 1Gel electrophoresis of nested PCR products for amplification of Toxoplasma gondii GRA6 gene. M: 100 bp molecular weight marker. Lane 1: positive control (Toxoplasma RH strain); lane 2: negative control (nuclease-free water); lanes 3, 4, 5, 7, and 8: positive nested PCR samples showed amplification at GRA6 gene-specific bands (791 bp). Lanes 6 and 9: negative samples.
Seropositivity of T. gondii infection in relation to risk factors among the patient (children with neurodevelopmental disorders) and control groups.
| Variable | Patient group ( | Control group ( | ||||||
|---|---|---|---|---|---|---|---|---|
| Tested | Positive | % | OR | Tested | Positive | % | OR (95% CI) | |
| Age group | ||||||||
| Neonate | 37 | 18 | 48.6 | 1.41 (0.53–3.71) | 31 | 4 | 12.9 | 0.64 (0.17–2.47) |
| Infant | 42 | 9 | 21.4 | 0.23 (0.03–1.85) | 50 | 7 | 14 | 0.47 (0.06–3.87) |
| Child | 101 | 37 | 36.7 | 0.79 (0.09–6.5) | 99 | 10 | 10.1 | 0.35 (0.04–2.88) |
|
| ||||||||
| Sex | ||||||||
| Male | 76 | 20 | 26.3 | 0.6 (0.17–2.47) | 82 | 9 | 11 | 0.97 (0.91–1.03) |
| Female | 104 | 44 | 42.3 | 98 | 12 | 12.2 | ||
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| Residence | ||||||||
| Urban | 48 | 8 | 16.7 | 4.3 (2.12–9.7) | 51 | 2 | 3.9 | 2.15 (1.06–4.39) |
| Rural | 132 | 56 | 42.4b | 129 | 19 | 14.7b | ||
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| Bottle feeding | ||||||||
| Yes | 38 | 9 | 23.7 | 0.63 (0.18–2.27) | 25 | 2 | 8 | 0.41 (0.04–4.63) |
| No | 142 | 55 | 38.7 | 155 | 19 | 12.2 | ||
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| Drink raw milk | ||||||||
| Yes | 30 | 5 | 16.7 | 0.20 (0.03–1.57) | 37 | 5 | 13.5 | 0.71 (0.15–3.26) |
| No | 150 | 59 | 39.3 | 143 | 16 | 11.2 | ||
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| Eating undercooked meat | ||||||||
| Yes | 34 | 7 | 20.6 | 0.59 (0.07–4.81) | 46 | 5 | 10.9 | 0.12 (0.02–0.92) |
| No | 146 | 57 | 39 | 134 | 16 | 11.9 | ||
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| Contact with soil | ||||||||
| Yes | 63 | 36 | 57.1b | 6.59 (3.2–13.7) | 46 | 9 | 19.6 | 1.28 (0.31–5.33) |
| No | 117 | 28 | 23.9 | 134 | 12 | 8.9 | ||
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| Contacts with cats | ||||||||
| Yes | 78 | 34 | 43.6a | 1.48 (0.57–3.8) | 79 | 11 | 13.9 | 1.11 (0.383–3.24) |
| No | 102 | 30 | 29.4 | 101 | 10 | 9.9 | ||
n: number of participants, OR (95% CI) : Odd Ratio (95% confidence interval), a: statistical significant at P < 0.05, b: statistical significant at P < 0.001, neonate <28 days old, infant: 28 days to 1 year old, child: 1–11 years old.
Seropositivity of T. gondii infection in relation to the neurodevelopmental disorders in the patient group.
| Neurodevelopmental disorders | Patient group ( | ||
|---|---|---|---|
| Tested | Positive | % | |
| Hydrocephalus | 26 | 18a | 69.2 |
| Microcephaly | 23 | 2 | 8.7 |
| Cerebral palsy | 44 | 6 | 13.6 |
| Epilepsy | 51 | 31b | 60.8 |
| Mental retardation | 16 | 2 | 12.5 |
| ADHD | 14 | 4 | 28.6 |
| Autism | 6 | 1 | 16.7 |
n: number of participants. aStatistical significant at P < 0.05. bStatistical significant at P < 0.001, ADHD: attention deficit hyperactive disorder.
Figure 2Agarose gel electrophoresis of MseI restriction enszyme digestion of Toxoplasma gondii GRA6 gene nested PCR amplification products. M: 100 bp molecular weight marker. Lanes 2, 3, 5, 7, 8, and 9: samples coinciding with type I (cutting bands at 168, 544 bp). Lanes 1, 4, and 6: atypical digestion pattern.
Toxoplasma gondii GRA6-RFLP genotypes in relation to neurodevelopmental disorders.
| Positive PCR cases ( |
| |
|---|---|---|
| Genotype I ( | Atypical pattern ( | |
| Hydrocephalus ( | 5 | 2 |
| Microcephaly ( | 2 | 0 |
| Cerebral palsy ( | 2 | 1 |
| Epilepsy ( | 5 | 0 |
| Mental retardation ( | 1 | 0 |
| ADHD ( | 1 | 1 |
n: number of patients, ADHD: attention deficit hyperactive disorder.