Risk factors for acquisition of scrub typhus in children admitted to a tertiary centre and its surrounding districts in South India: a case control study

The study period spanned 2 years from January 2015 to December 2016. Cases were children aged less than 15 years diagnosed to have scrub typhus at the Christian Medical College, Vellore (CMC) based on a positive InBiosScrub Typhus Detect™ IgM ELISA test (Inbios International Inc., Seattle, WA, USA) performed and interpreted as described previously [18]. Cases were included in the study if they resided within an 80 km radius of CMC and provided informed consent. Two age (+/− 1 year) and locality matched healthy controls were chosen for each case within a month of case recruitment. Age matching was done so that differences in behavioural patterns between ages are minimized. Location matching was done so that effect of differences in the macro-environment are negated. The house of the case was visited and closest street junction to the case’s house identified. A random number between 01 and 59 was then obtained to choose the control. The first digit denoted the direction of the street to be selected or a field hut (0-North, 1-East, 2-South, 3- West and 5- field hut). The second digit denoted the number of houses to be skipped in the chosen direction or the number of field huts to be skipped to choose a control. An age matched healthy control was then identified and chosen to take part in the study after obtaining informed consent. The same exercise was repeated to choose the second control. A recording form which included demographic, environmental and behavioural data was filled for both cases and controls. The recording form was filled by administering a questionnaire to a parent of the case or control and supplemented by a visual survey of the surroundings. Each control also had a blood sampling done for Scrub Typhus IgM and IgG to look for past or asymptomatic scrub typhus. All cases and controls houses were Geographic Information System (GIS) coded and plotted on a map to assess clustering. Socio-economic status scoring was done using the revised Kuppuswamy’s socio-economic status scale [19].

The potential risk factors assessed were determined by a pilot survey undertaken by two of the investigators. Sample size was calculated for a case to control ratio of 1:2 with the background exposure in controls expected to be 15%, to detect a factor with an odds ratio of 2 for cases with a 5% probability of type I error and 80% power. Ninety seven cases and 194 controls were needed.

The houses of all the cases in the case control study were visited by a field worker. Rodents and shrews were captured using Sherman traps of the size 3″ × 3″ × 10 ″ (W x H x L), designed for live capture of rats. The traps were baited with fried coconut. The traps were placed one hour before sunset and collected the next day morning. In each of the cases’ houses, 2 or 3 traps were placed inside and just around the houses. Once the rodent was trapped, the rodent was placed in a glass desiccator and a glass lid placed over the desiccator. Only one rodent was placed at a time in the desiccator. A single piece of unspun cotton was dipped in chloroform and then placed inside the glass desiccator. The animal is observed for cessation of voluntary movement and recumbency. A deep plane of anaesthesia was indicated by the lack of righting reflex when the container was tipped slightly and the respiratory rate was reduced to about 50% of the pre-anaesthetic rate (80–100 breaths/min). This usually happened in about 1 min in mice and 2 min in rats. If at any time the rodent had difficulty breathing (respiration becomes laboured, slows or stops), the desiccator was immediately opened and the rodent removed. Once the rodent was in deep plane of anaesthesia, it was removed from the desiccator and the animal’s mucous membrane colour, respiratory rate and withdrawal reflexes are checked. A noxious stimulus (toe pinch) was applied and if the animal responded to the toe pinch, it was returned to the desiccator for another 30 s. If the mucous membrane colour and respirations were normal and its withdrawal reflexes were absent, the rodent was ready for the mite collection. The ears and inter-digital spaces were swabbed with cotton tipped ear buds and the mite chiggers collected in an eppendorf tube with 70% alcohol. The hair was then combed on to a plastic tray and the mites collected in another eppendorf tube. If the rodents were trapped inside houses, they were released outside the house in the wild and if they were trapped outside, they were released back in the same place. Within a few minutes, the rodents were able to regain consciousness and run away. The eppendorf tubes were transported to the laboratory for identification of the mites and further testing. Mites were mounted in Hoyers medium, examined under the microscope and identified up to species level using standard taxonomical keys [20]. The chigger index (average number of chiggers per rodent) was estimated [21].

Ethics committee approval was obtained from the Institutional Review Board (Registration Number: ECR/326/INST/TN/2013 issued under Rule 122D of the Drugs & Cosmetics Rule 1945, Govt. of India) of Christian Medical College, Vellore to conduct the study. Institutional Animal Ethics Committee (IAEC) of the Christian Medical College, Vellore (Registration number: 88/PO/RcBi/SL/1999/CPCSEA registered with Committee for the Purpose of Control And Supervision of Experiments on Animals (CPCSEA), Ministry of Environment, Forests and Climate Change, Government of India) approval was also obtained for trapping of rodents to obtain mite chiggers. Written informed consent was obtained from a parent/guardian of all children who were enrolled in the study. Written assent was obtained from all children above the age of 8 years in addition to the parent/guardian consent. The rodents and shrews were captured using traps and anaesthetized to obtain mites from them. All rodents and shrews were released back in the same environment after obtaining the mites.