1. Introduction
Chickens represent the most numerous poultry species [1] and widely distributed in Nigeria [2]. Local chickens of the tropics are mainly kept for meat and egg production and sold sometimes for their socio-economic value [3]. One of the hot spots in chicken genetics and breeding research has been to identify major histocompatibility complex (MHC) haplotypes. Chen et al. [4] reported that MHC is a constellation of immune and immune-related genes involved in infectious disease prevention. It plays a fundamental role in both humoral and cellular immunity [5]. Thus, it is the most polymorphic loci in the chicken genome [6], containing two genetically-unlinked clusters; the B complex (MHC-B) and the restriction fragment pattern-Y (Rfp-Y) region [7]. The MHC-B contains the class I (BF), class IIβ (BLB), and extended class IV (BG) regions [8].
As reviewed by Han et al. [9], many approaches have been used to assess chicken MHC genotypes, including 2-dimensional electrophoresis, DNA random fragment length polymorphism (RFLP), single-strand conformation polymorphism, a genotyping method based on DNA sequence typing and red blood serological procedures. Serological procedure involving the use of sheep red blood cells (SRBC) have been used and reported in establishing some birds as chicken lines but such procedures have not been utilized in the Nigerian indigenous chicken. Ngongeh et al. [10] reported that there was evidence that resistance or susceptibility to some avian diseases was associated with inheritance and eventually, chicken lines resistant to such diseases could be established by genetic selection. No such documented evidence is known to the authors about the Nigerian indigenous (local) chicken in comparison to their exotic counterparts such as, broilers and layers where some related studies had already been conducted. Sheep red blood cell (SRBC) is an antigen that has been used to monitor immune response in chickens and has been used frequently as a potential antigen in immune response for it is non-pathogenic, strongly immunogenic and does not interfere with the measurement of antibody response [3].
The ability to simultaneously measure the transcript abundance of every known gene in a tissue sample opens the possibility of using gene expression as an intermediary molecular procedure to highlight genes governing a trait. Mapping of the encoding chicken genes suggests that BLB, the gene for MHC class II β chain, is a positional candidate gene [11]. BLB2 gene, pertaining to immune defense is regarded a major gene and expressed in a large variety of tissues in relatively high quantity in chickens [12]. Thus, the MHC is considered a barometer for the genetic health of species populations [13].
Data on the MHC class II and specifically BLB2 gene (classified as a major gene in immune defence) expression and characterisation in Nigerian indigenous chickens (NIC) therefore requires identification and proper elucidation of the immunological variation in the major genotypes (naked neck, frizzle and normal feathered chickens) based on quantitation indices. Thus, the alarming rate of loss of birds due to immune compromise at the point of disease attack which represents a substantial burden to farmers has evoked the need to study the precise mechanism of the immune protective mechanism via the BLB2 gene at the cytolytic and the latent stages in Nigerian indigenous chickens. Cytolytic response establishes after initial infection of birds followed immediately by a response phase that extends from 3 to 6 days post-infection [14]. Following cytolytic response, there is a switch to latent phase in T cells which occurs approximately 7 days post-infection [15].
2. Methods
2.1. Experimental Site
The study was carried out at the Poultry Unit of the Directorate of University Farms (DUFARMS), Animal Breeding and Genetics Departmental laboratory, the Biotechnology Centre Laboratory of the Federal University of Agriculture, Abeokuta and International Institute of Tropical Agriculture (IITA) Oyo State, Nigeria.
2.2. Experimental Animals
A total of 108 indigenous chickens were sourced across the six South-western states in Nigeria including Lagos, Ogun, Oyo, Osun, Ekiti and Ondo States, with 18 birds obtained per State, six (6) of each genotype of frizzle feather, naked neck and normal feather indigenous chickens and two (2) males and four (4) females. The birds were acclimatized and screened for diseases two weeks after sourcing. They were inoculated with sheep red blood cells (SRBC), after which blood samples were obtained from them (5 days post-inoculation) and antibody hemagglutination test was carried out to place the birds into groups of high and low antibody titres. One millilitre (1 ml) of washed 1% suspension SRBC antigen was intravenously administered to each of the birds. After 5 days post-injection, 1.5 ml of blood sample was collected from each bird via the jugular vein and was emptied into a non-heparinized bottle to induce clotting. Serum samples were separated from clotted blood and stored in eppendorf tube for hemagglutination test. Based on the result of the hemagglutination assay, birds from each genotype were grouped into high titre (≥9) and low titre (≤7) categories [16]. The categorisation of the birds into high and low titres resulted in six groups of two categories; high and low antibody titres. Hence, there were normal feather high, normal feather low, naked neck high, naked neck low, frizzle feather high and frizzle feather low antibody groups. Thereafter, artificial insemination was done to obtain progeny chicks. Semen from high titre males was used to inseminate high titre females and semen from low titre males was used to inseminate low titre females. Eggs generated from the birds were separated into different trays at the hatchery to avoid mixing up of birds after hatching.
2.3. Sample Collection
The chicks obtained across each group were sacrificed via cervical subluxation and dissected, commencing from eight weeks of age. Tissues (thymus and spleen) were subsequently removed aseptically, cleaned off, weighed (recorded) and placed in eppendorf tubes. Using blunt forceps, the tissues were teased apart immediately and stored in RNA latter to prevent degradation of the RNA prior to the time of extraction. This was thereafter stored in a −20˚C freezer, until the determination of the level of expression of the desired genes was carried out.
A total of 48 birds were isolated for surgical excision of thymus and spleen for detection of cytolytic and latent responses of the birds at eight (8) weeks. Cytolytic response detection in high and low titre chicks followed a selection of four birds (males and females) which were sacrificed for sample collection across the normal feather, naked neck and frizzle feather groups resulting in 24 birds. Latent response was detected in high and low titre birds by selecting two birds (male and female) which were sacrificed for sample collection across the normal feather low, naked neck low and frizzle feather low groups making a total of 24 birds. For cytolytic response, samples were obtained 5 days post-inoculation while for latent response, samples were obtained 14 days post-inoculation.
2.4. RNA Extraction and Quantitation Analysis
The total RNA of each tissue sample (thymus and spleen) was extracted using Isolate II RNA mini-kits (Bioline, London, UK) according to the manufacturer’s protocol. The primers used in the amplification of the BLB2 and β-actin genes were BLB2F (5'-CCCTCGGCGTTCTTCTTCTAC-3') and BLB2R (5'-CCCTCGG CGTTCTTCTTCTAC-3') and β-actinF (5'-GAGAAATTGTGCGTGACATCA-3') and β-actinR (5'-CCTGAACCTCTCATTGCCA-3') as reported by Lian et al. [17].
Two-step qPCR was conducted with the cDNA synthesis. Quantitation of reverse transcription product (cDNA) was achieved using SensiFASTTM SYBR Hi-ROX kit (Bioline, London, UK), using real time ABI 7500 machine which adopted two-step cycling; 1 cycle at 95˚C for 2 minutes (polymerase reaction) and 40 cycles at 95˚C for 5 seconds (denaturation) and 65˚C for 30 seconds (annealing/extension). The total reaction volume mixture used was 10 µl which included 2x SensiFAST SYBR Hi-ROX mix 5 µl, 0.5 µM forward primer, 0.5 µl reverse primer, 2.5 µl template cDNA and 1.5 µl water.
2.5. Statistical Analysis
The cycle threshold (Ct) from the qRT-PCR reactions of accumulated fluorescent signal curves was used to compute mean expression levels of the gene in tissues at different response phases and analysis of variance was conducted. Significant means were separated using least significant difference mean comparisons in R [18]. Interactions were not significant and thus unreported. The statistical model employed was:
where
= is the response/dependent variable
= is the overall mean response
= is the effect due to the ith genotype (i = normal feather, naked neck, frizzle)
= is the effect due to the jth antibody (j = high, low)
= is the effect due to the kth sex (k = male, female)
= is the effect due to the lth tissue (l = thymus, spleens)
= residual error
3. Results
The confirmation of presence of RNA after extraction from the tissue samples informed the choice of data analysis. Effects of tissue, genotype, antibody titre level and sex on the mean threshold cycle (CT) values of BLB2 gene expression of Nigerian indigenous chicken at cytolytic immune response stage are presented in Table 1. The results show that tissue (p < 0.001), titre grouping (p < 0.001) and sex (p < 0.01) significantly affected the mean expression of BLB2 gene at cytolytic immune response phase.
Table 1. Analysis of variance showing effects of tissue, genotype, titre and sex on BLB2 gene expression at the cytolytic stage of Nigerian indigenous chickens based on CT.
**p < 0.01, *** p < 0.001.
Table 2 shows separated ΔCT threshold means and fold difference (2−ΔΔCт) according to tissue, titre and sex at the cytolytic stage of Nigerian indigenous chickens. The result shows also that tissue (p < 0.001), titre grouping (p < 0.001) and sex (p < 0.01) significantly impacted the overall expression of BLB2 gene at cytolytic immune response phase.
The effects of tissue, genotype, titre and sex on the mean CT of BLB2 gene expression of Nigerian indigenous chickens at latent stage are presented in Table 3. The results show that tissue (p < 0.001), titre grouping (p < 0.01) and sex (p < 0.05) significantly affected the latent immune response phase.
Consequently, effects of tissue, genotype, titre and sex on ΔCT threshold means and the fold difference (2−ΔΔCт) of BLB2 gene expression of Nigerian indigenous chickens at latent stage is presented in Table 4. The result shows that tissue (p < 0.001), titre grouping (p < 0.01) and sex (p < 0.05) affected the latent immune response phase.
Table 2. Effects of tissue, titre, sex and genotype at the cytolytic gene expression in Nigerian indigenous chickens.
abcMeans in the same column within variable grouping bearing different subscripts are significantly different; SD—Standard Deviation; CT—Cycle threshold; ΔCт—Delta cycle threshold.
Table 3. Effects of tissue, genotype, titre and sex of latent gene expression of Nigerian indigenous chicken based on the CT threshold values.
**p < 0.01, ***p < 0.001; D.F—degree of freedom.
Table 4. Effects of tissue, titre, sex and genotype at the latent gene expression in Nigerian indigenous chickens.
abcMeans in the same column within variable grouping bearing different subscripts are significantly different; **p < 0.01, ***p < 0.001; SD—Standard Deviation; ΔCT—Delta cycle threshold.
4. Discussion
Tissue difference in CT values of spleen and thymus in the Nigerian indigenous chickens at cytolytic and latent immune response phases show that, average mean estimate for spleen and thymus at cytolytic phase was elevated. This result agrees with Patterson et al. [19] that CTs less than 29 are strong positive reactions indicative of abundant target nucleic acid in the sample. Birds categorised as having high titre estimates of immune response at the cytolytic stage had higher CT than at the latent phase, and this distinction was similar to the low immune response category. This finding conforms to the report by Le Blastier et al. [20] that CTs of 30 - 38 are moderate while CTs of 38 - 40 are weak reactions indicating minimal amounts of target nucleic acids. The result from this study suggests that higher mRNA content after extraction is an indication of marked deviation resulting from the low and high groups. Sarson et al. [21] reported that the CT of genes in the MHC-II pathway showed lower expression of genes of infected compared to uninfected chickens.
Observations from this study indicate that the CT values at the cytolytic phase were affected by tissue. Tissue expression of BLB2 gene considering 2−ΔΔCт represents the fold difference between the sample and the calibrator. The 2−ΔΔCт shows that the fold change of spleen at the cytolytic immune response of the birds was more profound (30,362.44) compared to the latent response (294.07). This could be due to the modulation of physiological manifestation of antigen response, which results in a burst of productive/restrictive infection in B cells that it is associated with high transcriptional activity of antigen at the cytolytic immune response stage which is followed by attraction and subsequent infection of thymus-derived CD4+ T cells at about 7 days post-infection. This finding is similar to the report of Heidari et al. [22] which verified an increase in physiological response in chicken following exposure to antigen in less than one week. Thymic expression was higher at the cytolytic phase compared to the latent phase of the high immune response birds than the low category. This result is congruent with the reports of Lian et al. [17] that the expression of genes in the MHC-IIpathway showed a decreased trend at all-time points in spleens of infected chickens compared to uninfected controls.
According to titre separation, 2−ΔΔCт values showed higher expression in birds categorised as high than in low counterparts at both the cytolytic and latent expression; and the fold difference on the overall. This observation is supported by the report of Xiaofei and Shannon [23] that experimental chicken lines would have a high possibility of multiple gene copy number per cell. Furthermore, the observation is in concord with the findings of Thanthrige-Don et al. [24] that there is significant down-regulation of MHC-II β-chain expression at 4, 14, and 21 days post-infection (d p.i.), and other components of the MHC-II heterotrimer (α chain and Ii chain) are also down-regulated at 4- and 21-days post-inoculation. Considering our results with the high and low categories at cytolytic immune response; and the same categories at the latent immune response, it could be inferred that the response of chicks of high-titre birds would most probably confer better survivability than the low-titre counterpart. Consequently, it would not be concluded that there was down-regulation considering the major gene BLB2 but repression. Heidari et al. [22] proposed that log fold change less than zero depicted down regulation and when the log fold values are greater than zero, it is not concluded as down-regulation.
Mean differences in the birds was also observed as the males had higher expression (2−ΔΔCт) estimates than females at both immuncompetence response stages. This observation conforms with the report of Zhao et al. [25] that nearly every cell in the body of chickens (from wattle to toe) has an inherent sex identity which is expressed; and in contrast with mammals, it demonstrates that avian somatic cells possess an inherent sex identity and as such, in birds, sexual differentiation is substantively cell-autonomous. In addition, it has been reported by Pierre [26] that both primary and secondary immune organs can be dramatically influenced by sex hormones.
5. Conclusion
At both cytolytic and latent stages of immune response to SRBC antigen, BLB2 expression in spleen was comparatively higher than thymus and the height of transcriptional activity was associated with the cytolytic stage. Consequently, according to antibody categorisation (high and low), birds of high titre at both cytolytic and latent responses had the highest mRNA expression. Nigerian indigenous birds of the male sex apparently had increased expression at cytolytic response stage at 8 weeks of age. During avian infections, it is proposed that the category of high immune response birds would most probably perform better than the low immune response counterpart. The use of SRBC to understand this phenomenon and the protective response BLB2 gene provides offer an understanding that the gene will be repressed from one time point to the other. It is important to note that mRNA levels documented in this report may not correlate with the amount of active protein expressed in vivo in the birds if there was post-translational modification of BLB2 product in the Nigerian indigenous chicken lines. It is therefore recommended that when considering diseases/infections responsible for substantial economic losses that plague the poultry industry, high response birds should be preferred. Also, for the purpose of commercial production, Nigerian indigenous chicken of the high immune response birds should be favoured. Studies should be carried out to compare the performance on the basis of immune traits to traits of economic importance (meat/body weight and egg production) and diseases.
Acknowledgements
This research was supported by Tertiary Education Trust Fund (TETFUND) Federal University of Agriculture, Abeokuta (FUNAAB). Special thanks to the Directorate of Grants Management FUNAAB.
Ethical Approval and Consent to Participate
All protocols for this research were approved by the Animal Care and Use Committee of the Federal University of Agriculture, Abeokuta, Nigeria.
Author’s Contribution
CONI, ASA and BIAA conceptualized and designed the study. BIAA collected the data and analyzed it. BIAA interpreted the results and drafted the manuscript and CONI supervised the study. MIT and ASA co-supervised and made critical revision of the manuscript. All authors have read and approved the manuscript.
Abbreviations
BLB2—B Locus Beta 2;
NIC—Nigerian indigenous chicken;
SD—Standard deviation;
CT—Cycle threshold;
ΔCT—Delta cycle threshold;
2−ΔΔCт—2(−Delta Delta cycle threshold).