Avian malaria and bird humoral immune response

To compare levels of humoral immune response of Plasmodium infected and uninfected birds under controlled conditions, canaries (Serinus canaria) were experimentally infected with Plasmodium relictum (lineage SGS1) in the laboratory. Thirty-two 1-year old canaries (15 females and 17 males) were kept in randomized groups of one to three individuals of the same sex per cage (1 × 1 × 2 m) in the animal facility (14:10 day–night light cycle, 20 °C, 55% humidity). Each of the 16 cages received fresh food (mix of 24 g of seeds, Vitabalance, and 18 g of couscous, Migros Bio) and fresh water (500 mL) daily, as well as a vitamin mix (Océvit, Virbac, 1 mL per litre of water) weekly. A first group of canaries (eight females and nine males) were experimentally infected via intra-peritoneal injection of 75 µL of a blood mix (prepared from blood of canaries previously infected with P. relictum) mixed with PBS (1:1). The control group (seven females and eight males) received an injection of the same volume of PBS. Once the infected canaries reached the chronic phase of infection (42 days post infection, hereby dpi, [24]), all the canaries were blood sampled and immune challenged (primary contact). At 49 dpi, they were blood sampled and immune challenged a second time (secondary contact). A final blood sample was taken at 56 dpi. Individuals were weighed prior to each blood sampling. The experiment was designed in two equivalent temporal blocks 1 week apart. After blood collection, haematocrit was measured in capillaries as the fraction of red blood cells in the total blood volume. The rest of the blood was centrifuged for 10 min at 4 °C at 15,000 relative centrifugal force. Plasma was stored at − 80 °C until immunological testing and red blood cells were stored at − 20 °C until Plasmodium detection and quantification.

In order to measure the bird humoral immune response when encountering a new pathogen, keyhole limpet haemocyanin (KLH), a molecule extracted from the giant keyhole limpet (Megathura crenulata) was used as an antigen. This molecule elicits a humoral immune response without pathogenic effects. A solution of KLH (Sigma-Aldrich) emulsified in PBS (1 mg/mL) and mixed with incomplete Freund’s adjuvant (Sigma-Aldrich, 1:1) was prepared according to [25]. Each bird received an intra-muscular (pectoral muscle) injection of 50 µL of KLH-adjuvant solution (25 µg of KLH per injection, adapted from [25]).

DNA was extracted from red blood cells using the DNeasy blood and tissue extraction kit (Qiagen) according to the manufacturer’s protocol for the BioSprint 96. A nested PCR was performed to detect the infection status of individuals. Following a primary reaction with the primers HaemNF1 and HaemNR3, a secondary reaction with the primers HaemF and HaemR2 to amplify Plasmodium was conducted as described in [26] adapted from [27] and 5 μL of PCR product was run on a 2% agarose gel to assess infection status.

Parasite quantification was performed by quantitative PCR as described in [26]. Briefly, two separate qPCR reactions using a parasite cyt b TaqMan probe (CY3-CYTb-BHQ2) and a host 18 s rRNA probe (FAM-18S-BHQ1) were performed. For both parasite and host, DNA concentration was calculated from the standard curve and the parasitaemia was given by the ratio of parasite DNA concentration on the host DNA concentration. In order to normalise the distribution, this ratio was log₁₀ transformed. As a consequence, we obtained a range of parasitaemia values increasing from − 2.10 to 1.10 (arbitrary unit) in infected canaries.

Statistical analyses were performed in R (version 3.1, [28]).

Anti-KLH antibody level was analysed as a response variable in linear mixed effect models (lme function in nlme package). Terms for sex (female–male), infection group (control–infected), antigen contact (primary–secondary contact) and all two-way interactions were included. Haematocrit and body mass were also analysed as response variables in linear mixed effect models including terms for sex (female–male), infection group (control–infected), antigen contact (prior to immune challenge—after primary contact—after secondary contact) and all two-way interactions. For Plasmodium infected canaries, parasitaemia over time was also investigated. Parasitaemia was analysed as a response variable in a linear mixed effect model including terms for sex, antigen contact (prior to immune challenge—after primary contact—after secondary contact) and their two-way interaction. Daily food consumption, calculated at the cage level, was analysed as a response variable in linear mixed effect models including terms for the density of canary per cage (1–3, to control for heterogeneity in the number of individuals per cage), sex (female–male), infection group (control–infected), time (as a quantitative continuous variable) and all two-way interactions between sex, infection group and time. Random factors were implemented as canary identity nested in cage nested in block (only cage nested in block for food consumption as it was calculated at the cage level) to account for the nested experimental design. An auto-correlation structure (corAR1) was implemented to account for repeated measurements. To determine the explanatory power of each fitted parameter, likelihood ratio tests were conducted following a standard backward selection procedure by sequential elimination of each fitted terms of similar order from the full model [29]. Only significant terms were kept to reach the minimal adequate model. The significant p values given in the text come from the minimal adequate models and the non-significant p values come from the likelihood ratio tests prior to the elimination of the non-significant term from the model. To look at the effect of each significant term individually, contrast analyses were performed [29].

As haematocrit is usually negatively affected by parasitaemia, the link between both parameters was also investigated. To account for the nested experimental design and repeated measurements, haematocrit was analysed as a response variable in a linear mixed effect model, implementing canary identity nested in cage nested in block as random factors and an auto-correlation structure (corAR1).