Paediatric Strongyloidiasis in Central Australia
Abstract
:1. Introduction
2. Review of Endemic Strongyloidiasis Epidemiology in Australia
3. Clinical Audit Methods
4. Results
5. Discussion
Ultimately, strongyloidiasis is a disease of poverty that reflects the appalling socioeconomic situation of Indigenous Australia. In some communities, a median number of 17 persons live in each house, and nearly 50% of dwellings do not have functioning facilities to remove faeces. The endemicity of both S. stercoralis and HTLV-1... renders public education and improvements to housing imperative.
6. Conclusions
Author Contributions
Conflicts of Interest
References
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Author | Location | Sample Size and Demographics | Years Studied | Diagnostic Test | Key Findings |
---|---|---|---|---|---|
Frith et al., 1974 [26] | NSW: Central Coast | Not stated | 1966–1967 | Stool examination | 4.7% positive on stool microscopy |
Jones, 1980 [26] | WA: 20 remote communities | 1683 adults and children | 1973–1978 | Stool microscopy with formol-ether concentration | 2% positive on faecal microscopy Highest infection rate in 15–19 year old age group |
Prociv and Luke, 1993 [27] | QLD: 122 remote communities | Children <15 years providing 32,145 faecal samples for diagnosis and disease surveillance | 1972–1991 | Stool microscopy with formol-ether concentration | Overall infection prevalence of 1.97% positive Cases found in 52/122 communities Peak prevalence of 27.5% in one area during wet season vs average prevalence of 12% Reduction in prevalence from 26.2% to 7% with thiabendazole treatment of infected children |
Meloni et al., 1993 [12] | WA: Kimberly region | 247 adults and children in five communities | 1987–1991 | Stool examination | 0.25% positive on microscopy 0.3% in children aged 0 to 13 |
Gunzburg et al., 1992 [32] | WA: Kimberly region | 104 Indigenous children under 5 years old | Not stated | Stool concentration and microscopy | 1.2% of samples from children with diarrhoea and 2.1% of samples from well children positive |
Fisher et al., 1993 [13] | NT: Darwin | ~2000 stool samples from adult and paediatric patients | 1991–1992 | Stool examination | 68 cases of S. stercoralis identified 54% of diagnoses were in children under 5 years Eosinophilia noted in 57% of cases |
Yiannakou et al., 1992 [33] | QLD: Townsville | 14 adult and paediatric cases from 5 year audit | Not stated | Stool examination | 9 Indigenous cases, 2 refugees from Vietnam, 1 returned veteran and 2 non-Indigenous patients with no significant travel history |
Flannery and White, 1993 [30] | NT: Arnhem Land | 29 participants | Not stated | Single stool microscopy; Serology | 41% positive on faecal microscopy 59.6% positive by serological diagnosis |
Shield et al., 2015 [15] | NT: Arnhem Land | 314 participants including 129 children; 39 underwent serology | 1994–1996 | Stool microscopy; Serology | 19% positive on microscopy 28% seropositive and 18% equivocal |
Aland et al., 1996 [11] | NT: Arnhem Land | 300 participants | Not stated | Single stool microscopy | 15% positive on faecal microscopy |
Page et al., 2006 [34] | NT: Arnhem Land | 508 adult and adolescent participants | 1996–2002 | Serology | 35% positive by serological diagnosis at baseline 78% seroreversion rate of cases with treatment |
Kukuruzovic et al., 2002 [14] | NT: Darwin | 291 children admitted with diarrhoea and 84 controls | 1998–2000 | Stool examination | 7.2% of stool samples had S. stercoralis detected 87 children with wasting were 6.5 times (95% CI 1.6 to 26.7) more likely to have S. stercoralis Hypokalaemia significantly associated with S. stercoralis infection |
Einsiedel et al., 2008 [35] | NT: Alice Springs | 206 Indigenous adults admitted with blood stream infections | 2001–2005 | Serology | 35.4% were positive by serological diagnosis |
Einsiedel and Fernandez, 2008 [5] | NT: Alice Springs | 18 Indigenous adults admitted with severe strongyloidiasis | 2000–2006 | Stool examination; Serology | 7/11 patients with severe disease tested for HTLV-1 were positive |
Einsiedel et al., 2014 [20] | NT: Alice Springs | 1126 Indigenous adult inpatients | 2000–2010 | Serology | 23.9% positive by serological diagnosis HTLV-1 positive patients trending towards higher seropositivity rates but not significant (p = 0.063) |
Mayer-Coverdale et al., 2017 [9] | NT: Territory-wide | 22,892 adult and paediatric stool samples provided to NT pathology services | 2002–2012 | Microscopy with formol-ether concentration | 97.7% of cases Indigenous, overall 1.7% positive 42.2% of diagnoses in children under 5 years of age (3–6% positive) Declining rates of diagnosis over time noted |
Kearns et al., 2017 [16] | NT: Arnhem Land | 859 Indigenous children and adults | 2010–2011 | Microscopy/culture; Serology | 21% seropositive at baseline with 15% equivocal Peak seropositivity in 5–14 year old cohort 89% patients had eosinophilia at baseline 11% had positive faecal microscopy/culture Seroprevalence 2% at 18 months after two mass drug administrations |
Hays et al., 2015 [36] | WA: Kimberly region | 259 Indigenous adults | 2012–2015 | Serology | 35.3% positive by serological diagnosis (OD > 0.3) Reduction to 5.8% after three years of targeted treatment and follow up of seropositive patients |
Variable | Seronegative (n = 156) Number (%) | Seropositive (n = 30) Number (%) | p Value |
---|---|---|---|
Mean Age | 6 years 1 month | 6 years 7 months | p = 0.55 |
Male Gender | 91 (58.3%) | 22 (73.3%) | p = 0.12 |
Remote | 109 (69.9%) | 27 (90.0%) | p = 0.02 |
Indigenous | 149 (95.5%) | 30 (100%) | p = 0.24 |
Mean serology | N/A | Optic density = 0.84 ± 1.54 | |
Stool pathogens | 17 (36.2%), n = 47 | 5 (62.5%), n = 8 | p = 0.16 |
Haemoglobin | 117.63 ± 25.92 g/L | 116.77 ± 27.22 g/L | p = 0.74 |
Mean corpuscular volume | 76.578 ± 10.18 fL | 76.66 ± 7.72 fL | p = 0.93 |
Mean eosinophil count * | 0.96 × 109/L ± 2.13 × 109/L (Range 0.5 × 109/L to 5.3 × 109/L) | 1.83 × 109/L ± 1.32 × 109/L (Range 0.6 × 109/L to 4.8 × 109/L) | p < 0.0001 |
Gastrointestinal symptoms | 40 (25.6%) | 9 (30%) | p = 0.62 |
Respiratory symptoms | 42 (26.9%) | 7 (23.3%) | p = 0.68 |
Blood stream infection | 4 (2.6%) | 0 (0%) | p = 0.37 |
Growth faltering | 25 (16%) | 3 (10%) | p = 0.4 |
HTLV-1 seroprevalence | 0/10 (0%) | 0/2 (0%) |
Seronegative (n = 47/156) Number (%) | Seropositive (n = 8/30) Number (%) | |
---|---|---|
Organism/virus identified | 17 (36%) | 5 (62.5%) |
Strongyloides stercoralis | 0 | 0 |
Giardia species | 5 | 2 |
Cryptosporidium parvum | 3 | 2 |
Blastocystis hominis * | 1 | 0 |
Trichomonas hominis ** | 1 | 0 |
Entamoeba coli ** | 1 | 0 |
Entamoeba hartmanni ** | 1 | 0 |
Salmonella species | 3 | 0 |
Campylobacter jejuni | 1 | 0 |
Norovirus | 4 | 0 |
Rotavirus | 1 | 0 |
Adenovirus | 1 | 2 |
Hymenolepis nana | 1 | 0 |
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Wilson, A.; Fearon, D. Paediatric Strongyloidiasis in Central Australia. Trop. Med. Infect. Dis. 2018, 3, 64. https://doi.org/10.3390/tropicalmed3020064
Wilson A, Fearon D. Paediatric Strongyloidiasis in Central Australia. Tropical Medicine and Infectious Disease. 2018; 3(2):64. https://doi.org/10.3390/tropicalmed3020064
Chicago/Turabian StyleWilson, Angela, and Deborah Fearon. 2018. "Paediatric Strongyloidiasis in Central Australia" Tropical Medicine and Infectious Disease 3, no. 2: 64. https://doi.org/10.3390/tropicalmed3020064
APA StyleWilson, A., & Fearon, D. (2018). Paediatric Strongyloidiasis in Central Australia. Tropical Medicine and Infectious Disease, 3(2), 64. https://doi.org/10.3390/tropicalmed3020064