Mitochondrial Cyt-b and Cox1 Genes Based Molecular Diversity and Phylogenetic Analysis of Chukar Partridge (Alectoris chukar)
Mitochondrial Cyt-b and Cox1 Genes Based Molecular Diversity and Phylogenetic Analysis of Chukar Partridge (Alectoris chukar)
Maria Khalid1, Tanveer Hussain1*, Zahid Farooq2, Kamran Abbas1 and Masroor Ellahi Babar1
1Department of Molecular Biology, Virtual University of Pakistan, Lahore
2The Cholistan University of Veterinary and Animal Sciences, Bahawalpur
ABSTRACT
The taxonomy of Alectoris chukar (A. chukar) has been a complex debate with different classifications and revisions suggested based on their morphology, geographical distribution and chromosome number. In Pakistan the Chukar partridge (A.chukar)), is an important member of Phasianidae family, however a scarce molecular data is reported that urged us to investigate its genetic diversity and phylogeny using mitochondrial DNA, Cyt-b and Cox1 genes. A total of 749bp of Cox1 and 472 bp of Cyt-b complete coding regions of both genes were amplified by PCR followed by sequencing. The sequences were aligned and edited using Bio-Edit software and single nucleotide polymorphisms (SNPs) were identified. The boot strapped Neighbor joining tree constructed from MEGA7 explained the genetic relationships of A.chukar with related members of Phasianidae family. The phylogenetic analysis also showed the genetic positioning of A. chukar with respect to other different reported species as well. The study gave us useful genomic information about genetic diversity in A. chukar and its phylogenetic relationships with related taxa, emphasizing on need of execution of conservation strategies to protect this unique genetic resource of Pakistan.
Article Information
Received 11 October 2018
Revised 02 March 2019
Accepted 03 May 2019
Available online 1 May 2020
Authors’ Contribution
MK and ZF collected blood samples and perfumed PCR. KA and TH helped in PCR and data analysis. MK and KA wrote the article.
Key words
Chukar, Cyt-b, COX1, Phylogenetic, PCR
DOI: https://dx.doi.org/10.17582/journal.pjz/20181011191004
* Corresponding author: [email protected]
0030-9923/2020/0004-1607 $ 9.00/0
Copyright 2020 Zoological Society of Pakistan
Chukar Partridge (Alectoris chukar) is national bird of Pakistan. This 13-15 inches long medium sized bird (Nowaczewski et al., 2014) belongs to family Phasianidae (Kerr et al., 2009; Shen et al., 2010; Sutherland et al., 2004) consisting of 16 reported sub species (Song and Liu, 2013). A. chukar shows most similarity to Alectoris rufa (also known as red- legged partridge) which exists in Western areas of the world (Barbanera et al., 2007; Christensen, 1996). Worldwide it is present in Palestine, Turkey, Iran, Lebanon, India, Central Nepal, Middle East, Afghanistan, Pakistan, Western Himalayas, Europe, Africa, Israel, Jordan and Dead Sea area (Grewal and Bhatia, 2017; Whistler, 2007; Baker, 1928). In Pakistan it is distributed in Sindh, Salt Range, Chitral, Swat, Kohistan, Gilgit, Punjab, Baluchistan, Sindh and Azad Jammu Kashmir (Pathan et al., 2014). According to North American Breeding Bird Survey, Chukar populations have been stable and are slightly increasing, since being introduced into North America (Christensen, 1996) so it’s at the status of Least Concern (LC) (IUCN Red-list 2010) and there are no widespread conservation measures in place for this bird (Bird Life International). But for Pakistan its importance being our unique genetic national resource cannot be denied.
mtDNA has many advantageous reasons to be chosen above other markers for phylogenetic analysis and molecular diversity studies (Hussain et al., 2015). In this study we explored mitochondrial Cyt-b and Cox1 genes in A. chukar from different locations of Pakistan to have insight about its genetic architecture by measuring polymorphism and phylogenetic relationships within A. chukar and related Phasianidae family members.
Materials and methods
Blood samples (n=30) were collected from A.chukar of Bahawalpur Zoo and Gatwala Wildlife Park Faisalabad with the support and permission from Pakistan Wildlife Foundation (PWF). The DNA was extracted using standard organic method (Sambrook and Russell, 2006) DNA samples concentration was measured using gel electrophoresis.
A specific pair of primers for Cytb-Fw5’TACCATGAGGACAAATATCATTCTG Rev5’ CCTCCTAGTTTGTTAGGGATTGATCG) was taken from Naseer et al. (2018) and Cox1-Fw5’TCTCAACCAACCACAARGAYATYGG Rev5’TAGACTTCTGGGTGGCCRAARAAYCA was taken from Hassanin et al. (2012). The amplified 472bp product was for Cyt-b and 749bp for Cox1.
For the amplification of mitochondrial Cyt-b and Cox1 genes the PCR was carried out using BioRad (USA) thermocycler in a reaction volume of 25 μl containing genomic DNA, PCR buffer, dNTPs, MgCl2, forward and reverse primers, Taq DNA polymerase (BioRon , Germany)and nuclease-free water. The conditions used were for Cyt-b: initial denaturation 95˚C for 5 min, followed by 5 cycles of 95˚C for 45 sec; 45˚C for 1 min 72˚C for 1 min, then 30 cycles of 95˚C for 45 sec, 48oC for 1min and 72˚C for 1 min and final extension at 72˚C for 10 min. For Cox1: initial denaturation 94˚C for 3 min, followed by 10 cycles (with 1 oC decrease in each cycle) of 94˚C for 1 min; 65˚C for 1 min and 72˚C for 1 min, then 25 cycles of 94˚C for 1 min, 55oC for 1min and 72˚C for 1 min and final extension at 72˚C for 7 min. The PCR products (3 μL of PCR product and 2μL of loading dye mixed) were run on 1.2 % Agarose gel at 90 Voltages for 35 min in 1X TAE buffer and seen by gel documentation system (Bio Rad, USA) under UV light. The positive samples were sent for sequencing to 1st Base Laboratories Singapore. The obtained sequences were aligned with the help of online NCBI BLAST (http/www.ncbi.nlm.nih.com) to see relevant reported sequences. The sequences were edited and assembled through Bio-Edit software (Hall, 1999) for the identification of single nucleotide polymorphisms. DnaSP v. 5software (Librado and Rozas, 2009) was used to reconfirm SNPs and to observe haplotypes. MEGA7 program package was used (Tamura et al., 2013) to construct Neighbor-Joining (Saitou and Nei, 1987) evolutionary trees ((1000 bootstrap value) for Alectoris chukar and other the related taxa assembled together are shown next to the branch as a percentage of replicate trees (Felsenstein, 1985). The Maximum Composite Likelihood method was used to calculate evolutionary distances (Tamura et al., 2004) and are in the units of the number of base substitutions per site.
Results
SNPs were identified by using DnaSP (Librado and Rozas, 2009) in Alectoris chukar in 423bp and 599 bp of Cyt-b and Cox1 respectively. In Cyt-b there were 412 invariable (monomorphic) sites while variable (polymorphic) sites found are only 11 (53, 56, 86, 94, 124, 136, 161, 190, 198, 258, 271) which were all parsimony informative sites with two variants and there was no Singleton variable site. In Cox1 there were 517 invariable (monomorphic) sites while 73 variable (polymorphic) were observed out of which 61 were Singleton variable sites, 12 Parsimony informative sites. (Table I).
Table I. Single nucleotide polymorphisms (SNPs) identified in 599 bp fragment of Cox1 in 20 samples of Alectoris chukar.
Nucleotide Position |
Variation |
2, 3, 4, 8, 11, 21, 22, 30, 53, 56, 57, 63, 64, 66, 69, 73, 78, 81, 86, 93, 99, 103, 112, 114, 117, 142, 144, 149, 152, 157, 161, 166, 168, 169, 178, 194, 195, 197, 199, 208, 224, 228, 256, 258, 261, 271, 274, 276, 303, 330, 445, 484, 554, 574, 575, 577, 587, 589, 590, 593. |
Singleton variable sites of (two variants) |
7, 14, 15, 27, 34, 39, 128, 198, 200, 211, 223 |
Parsimony informative sites (two variants) |
44 |
Singleton variable sites (three variants) |
192 |
Parsimony informative sites (three variants) |
In Alectoris chukar for Cyt-b gene 11 haplotypes (h) with 1.0000 haplotype (gene) diversity (hd) , variance of Haplotype diversity was found 0.00150, with standard deviation of 0.039, and per site nucleotide diversity (Pi) 0.49587, The sampling variance of Pi was calculated as 0.0016083 and standard deviation of Pi was 0.04010 and in Cox1 gene 10 haplotypes (h) with 0.711 haplotype (gene) diversity (hd), variance of haplotype diversity was found 0.01288, with standard deviation of 0.113 and per site nucleotide diversity (Pi) 0.01509, The sampling variance of Pi was calculated as 0.0000476 and standard deviation of Pi was 0.00690.
For Cyt-b the overall genetic distance among all Alectoris chukar sequences 0.0142. The evolutionary history was inferred using the neighbor-Joining method. The optimal tree with the sum of branch length = 0.04688547 (Supplementary Fig. 1). For Cox1 the overall genetic distance among all Alectoris chukar sequences 0.0147. Optimal branch length of the tree is 0.41892384 (Supplementary Fig. 2). The trees were drawn to scale, with branch lengths in the same units as those of the evolutionary distances used to infer the phylogenetic tree. The evolutionary distances were computed using the Maximum Composite Likelihood method and are in the units of the number of base substitutions per site. The genetic distance comparison between sample Chukars and other sequences in Phasianidae family obtained from NCBI was performed for both Cox1 and Cytb genes. The analysis showed that for Cytb there is 90% to 99% (Table II) similarity amongst sample sequences and for Cox 1 there is 93% to 100 % similarity observed (Table II).
Table II. Comparison of Alectoris chukar samples sequences with sequences of Phasianidae family available in NCBI for Cyt-b and Cox1.
Samples |
Similarity (%) |
Accession # |
Cyt-b |
||
A. chukar _ 1_Cytochrome b |
95% |
GU214294.1 |
A. chukar _ 2_Cytochrome b |
99% |
KY829450.1 |
A. chukar _ 3_Cytochrome b |
94% |
AM850828.1 |
A. chukar _ 4_Cytochrome b |
93% |
FJ752426.1 |
A. chukar _ 5_Cytochrome b |
99% |
GU214293.1 |
A. chukar _ 6_Cytochrome b |
98% |
GU214292.1 |
A. chukar _ 7_Cytochrome b |
94% |
AM850784.1 |
A. chukar _ 8_Cytochrome b |
93% |
AM850752.1 |
A. chukar _ 9_Cytochrome b |
97% |
EU893475.1 |
A. chukar _ 10_Cytochrome b |
96% |
AM850788.1 |
A. chukar _ 11_Cytochrome b |
90% |
AM850752.1 |
Cox1 |
||
Chukar_1_Cox1 |
99% |
KY829450.1 |
Chukar_2_Cox1 |
97% |
KT806484.1 |
Chukar_3_Cox1 |
93% |
JF498827.1 |
Chukar_4_Cox1 |
99% |
JF498826.1 |
Chukar_5_Cox1 |
99% |
GQ481315.1 |
Chukar_6_Cox1 |
99% |
DQ432706.1 |
Chukar_7_Cox1 |
99% |
AY666409.1 |
Chukar_8_Cox1 |
98% |
GU951807.1 |
Chukar_9_Cox1 |
99% |
FJ808621.1 |
Chukar_10_Cox1 |
99% |
KT803621.1 |
Chukar_11_Cox1 |
99% |
GQ481314.1 |
Chukar_12_Cox1 |
99% |
AY666409.1 |
Chukar_13_Cox1 |
99% |
JF498828.1 |
Chukar_14_Cox1 |
100% |
DQ432706.1 |
Chukar_15_Cox1 |
98% |
FJ465298.1 |
Chukar_16_Cox1 |
99% |
KT806484.1 |
Chukar_17_Cox1 |
100% |
DQ432706.1 |
Chukar_18_Cox1 |
99% |
JF498827.1 |
Chukar_19_Cox1 |
99% |
KT803621.1 |
Chukar_20_Cox1 |
100% |
DQ432706.1 |
Discussion
According to North American Breeding Bird Survey, Chukar populations have been stable and are slightly increasing, since being introduced into North America (Christensen, 1996). Although in some areas it has been affected by habitat destruction, for example in Azerbaijan. In Turkey it has been affected due to pesticide usage, while in USA and Canada hunters and poachers can be a source of discomfort for this bird (McCarthy, 2006). Overall in world it has a large range and stable population, so is not currently considered to be at risk of extinction. Chukar has a status of Least Concern (LC) according to International Union of Conservation of Nature (IUCN Red-list 2016) and there are no widespread conservation measures in place for this bird some proposed conservation actions include assessment of the impacts of pesticides on this species and identification of key areas of habitat for this species to be introduced, protected and expanded. Chukar is our National Bird so it has a significant importance and its conservation for future is need of our country.
In the past, this important bird has not been considered for its characterization and evaluation level at which this study has been conducted. Previously mtDNA has been widely used to investigate closely related animals (Achilli et al., 2012; Achilli et al., 2009). Here, DNA samples of several species were isolated and the molecular diversity and phylogenetic were explored using Cyt-b and Cox1 mitochondrial genes in Alectoris chukar from different areas of Pakistan. The phylogenetic analysis showed that Chukar have adapted to the environment independently according to their unique capacity which represents that they have achieved lineage specific variations in that particular genetic region.
Conclusion
As being national bird of Pakistan, Chukar must be considered as a rare animal to get attention for suitable conservation actions. This study demonstrates the genetic diversification and phylogenetic differentiations of this unique bird. Our study provided useful material for supporting conservation strategies and breeding plans for this important bird, however further genomic investigations should be carried out at larger scale.
Acknowledgements
A special thanks to Punjab Wildlife Department for helping in blood sampling.
There is supplementary material associated with this article. Access the material online at: https://dx.doi.org/10.17582/journal.pjz/20181011191004
Statement of conflict of Interest
The authors have declared no conflict of interest.
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