key: cord-1036604-kifsxqq2 authors: Li, Hui; Wang, Jia-Xin; Wu, Dong-Dong; Wang, Hua-Wei; Tang, Nelson Leung-Sang; Zhang, Ya-Ping title: The Origin and Evolution of Variable Number Tandem Repeat of CLEC4M Gene in the Global Human Population date: 2012-01-18 journal: PLoS One DOI: 10.1371/journal.pone.0030268 sha: 28b64c3ea5c13cbcaae132a45661fb8bf5c25c62 doc_id: 1036604 cord_uid: kifsxqq2 CLEC4M is a C-type lectin gene serving as cell adhesion receptor and pathogen recognition receptor. It recognizes several pathogens of important public health concern. In particular, a highly polymorphic variable number tandem repeat (VNTR) at the neck-region of CLEC4M had been associated with genetic predisposition to some infectious diseases. To gain insight into the origin and evolution of this VNTR in CLEC4M, we studied 21 Africans, 20 Middle Easterns, 35 Europeans, 38 Asians, 13 Oceania, and 18 Americans (a total of 290 chromosomes) from the (Human Genome Diversity Panel) HGDP-CEPH panel; these samples covered most of alleles of this VNTR locus present in human populations. We identified a limited number of haplotypes among the basic repeat subunits that is 69 base pairs in length. Only 8 haplotypes were found. Their sequence identities were determined in the 290 chromosomes. VNTR alleles of different repeat length (from 4 to 9 repeats) were analyzed for composition and orientation of these subunits. Our results showed that the subunit configuration of the same repeat number of VNTR locus from different populations were, in fact, virtually identical. It implies that most of the VNTR alleles existed before dispersion of modern humans outside Africa. Further analyses indicate that the present diversity profile of this locus in worldwide populations is generated from the effect of migration of different tribes and neutral evolution. Our findings do not support the hypothesis that the origin of the VNTR alleles were arisen by independent (separate) mutation events and caused by differential allele advantage and natural selection as suggested by previous report based on SNP data. Dendritic cell-specific intracellular adhesion molecular-3grabbing nonintegrin (CLEC4L) and L-SIGN also called DC-SIGN related (CLEC4M) are C-type lectins involved in both innate and adaptive immunity. They are cell adhesion receptors and pathogen recognition receptors. However, CLEC4L (also called CD209) is expressed primarily on phagocytic cells, such as dendritic cells and macrophages, whereas CLEC4M (also called CD209L) expression is restricted to endothelial cells in liver and lymph nodes [1, 2] . Both lectins are known to bind multiple pathogens and function as cellular receptors for various viruses, such as HIV-1, Ebola virus, cytomegalovirus, hepatitis C virus, Dengue virus, and SARS-coronavirus [3] [4] [5] . With regards to CLEC4M, it serves as a receptor for a variety of viruses, including HIV-1, hepatitis C, Ebola, and SARS-coronavirus, as well as the parasite Schistosoma mansoni and bacteria Mycobacterium tuberculosis [6, 7] . These two lectins are coded by genes that are located within a lectin family genes cluster on chromosome 19p13.2-3. This 26-kb segment is believed to arise as a result of a duplication of an ancestral gene [8] . These two genes in the cluster share a high degree of homology [2] . Both proteins are organized into three domains: (1) an N-terminal cytoplasmic region with a di-leucine motif for internalization followed by a transmembrane domain, (2) a C-terminal extracellular domain with a C-type carbohydrate recognition domain (CRD) involved in pathogen binding, and (3) a neckregion containing variable number of repeats of conserved subunit of 23-amino-acid sequence, that connects the CRD to the transmembrane region. The neck-region is involved in assembling the lectin into a tetrameric protein conformation on the cell surface, which is believed to be required for efficient recognition of multivalent ligands. And the length variation of this neck-region had been proposed to affect the pathogen-binding properties of the CRD of these proteins [9, 10] . However, this property is controversial [9] . Genetic association studies also showed conflicting results about the associations of length variation of neck-region and several infectious diseases, such as HIV, HCV, and SARS [11] [12] [13] [14] [15] [16] [17] [18] [19] . CLEC4M neck-region exhibits a higher level of heterozygosity due to presence of 4-to 9-repeats in substantial frequencies in the populations. On the other hand, the VNTR in CLEC4L is highly conserved (7 repeats is found in .90% in the population). Previous study showed that CLEC4L had been under a strong selective constraint, while CLEC4M had been shaped by the action of balancing selection, and the VNTR region of these two genes might be the target of such selective pressures [20] . The VNTR repeat length polymorphism in CLEC4M has been suggested to be associated with genetic predisposition to infection. We investigated the origin and evolutionary history of this VNTR in human population by clonal sequencing. Samples from the Human Genome Diversity Panel (HGDP)-CEPH panel of different continents were studied. The HGDP-CEPH panel is a resource of 1064 cultured lymphoblastoid cell lines (LCLs) from individuals in 52 different world populations. Information for each LCL is limited to sex, population, and geographic origin of the individual. The panel contains LCLs from populations living on all continents and is collected to provide unlimited supplies of DNA for studies of sequence diversity and history of modern human populations [21] . The sequence identity of each repeat subunit of different VNTR alleles are identified by sequencing after cloning the PCR product and the haplotype structure including identity of each subunit and their orientation of each VNTR (from 4 to 9 repeats) is thus determined. Our results showed that the haplotype of subunits of the same VNTR (from 4 to 9 repeats) sampled from subjects of different continents were virtually identical, which implied the different VNTR alleles in CLEC4M gene had existed for a long time, at least before the date of ''out-of-Africa'' event. Furthermore, by using the genotype data of VNTR in CLEC4M gene and dividing the subjects of the Human Genome Diversity Panel (HGDP)-CEPH panel into 26 populations, we analyzed the correlation between the 25 non-African populations geographic distance to the east Africa and their population genetic distance to the east Africa. We concluded that the present diversity profile of this VNTR in worldwide populations was consistent with demographic migrating of different tribes. No evidence was found to support the notion of independent mutation events due to natural selection. Sequence identity of the subunits in VNTR of CLEC4M Gene Work by our team and others showed that the VNTR in CLEC4M gene varied in size from 4 to 9 repeats [18] . In this study, we analyzed the sequence identity of each subunit among VNTR of 4 to 9 repeats alleles of 145 samples from different continental populations by clonal sequencing. Figure 1 shows the various haplotypes of each subunit and the prevalent subunit orientation in each VNTR alleles. Only eight different haplotypes account for all sequence variations of all subunits. H2 is the most parsimony one and thus used as the consensus sequence. According to the sequence identity in the 69-bp repeat unit, seven other haplotypes are identified (denoted as H1-H8) ( Figure 1 ). Different numbers of these subunits assemble to form the VNTR alleles of different length. The most prevalent subunit structures of each VNTR are described in Figure 2 . The detailed haplotype configurations in VNTR locus for all studied samples are found in Table S1 . In most VNTR, the N-terminal repeat unit (H1) and C-terminal repeat unit (H4 followed by H5) are highly conserved. Most alleles has H1 and H4 followed by H5 (or their transition variants) in these two locations ( Figure 2 ), which is supportive that these subunits are important for the formation of oligomer of CLEC4M [9] . As the 7-repeat allele is the dominant allele in worldwide population, we used the sequencing result of this 7-repeat haplotype as an illustration. One hundred and thirteen alleles of the 7-repeat were sequenced, and 96.5% of them showed identical haplotype and arrangement of subunits. On the direction from the N-terminal to C-terminal, the 7-repeat allele is formed by one H1, three H2, one H3, one H4 and one H5. Thus, it is denoted as H1-H2-H2-H2-H3-H4-H5 in the table of supplementary data (Table S1) , and this construction is defined as the common consensus configuration. The consensus configurations of other VNTR alleles are also shown in table 1. For 7-repeat allele, the remainder has one of the three variant configurations which accounted for less than 4%. These variants are due to replacement of one of the H2 subunit by H3 subunit or vice versa. As H2 subunit and H3 subunit differs by three base pairs, it is not caused by a single sporadic event. They represent a signal of independent origin in a small proportion of 7-repeat allele. Therefore, these variants of 7repeat are classified as major rearrangement in Table 1 . When the longer repeat alleles were compared with the shorter one, it is apparent that the expansion of VNTR is due to insertion of H2 subunit (e.g. 8-repeat and 9-repeat). On the other hand, shorter repeat alleles were formed by deletion of H2 subunit. The 7-repeat was the dominant allele and was composed of five haplotype subunits in between the terminal subunits ( Figure 2 ). The 6-repeat, 8-repeat and 9-repeat, had the same haplotype subunit order as the 7-repeat, except for loss or duplication of the subunit H2 (Figure 2) . A dominant consensus configuration can be found in most VNTR alleles. Table 1 shows that only less than 2.5% of the alleles have a major rearrangement. It is found that an independent Table 1 . The proportion of the common consensus configuration, minor variant and major rearrangement in VNTR. Note: minor variant: the difference between two subunits is due to a single base change which also represents a transition change. major rearrangement: change from one subunit haplotype to another with difference in multiple base pairs or a change in the order of subunits. It signifies that the rearrangement cannot be caused by a single sporadic mutation. It may represent an independent origin of the alleles and candidates for natural selection. doi:10.1371/journal.pone.0030268.t001 origin as reflected by prevalence of major rearrangement in a repeat allele was more frequent (6.6%) in the longest allele (9repeat), suggesting that the longest allele may be found by separate mutagenesis events. On the other hand, all other alleles have only one dominant consensus configuration, together with minor variants of single base transition change which may be due to sporadic transition events. In general, the haplotype subunit and their configuration in each VNTR alleles are common in populations across different continents, and it suggests that they should be originated before the out-of-Africa event, and maintained for a long time. Barreiro et al. have reported that using data of adjacent SNPs of the locus, the CLEC4M gene evolved under balancing selection in non-African populations and pointed out that the neck-region was the functional target of such selection [20] . However, we showed that a different mechanism, namely demographic migration might explain equally well the generation of the VNTR diversity based on the sequence subunits within the VNTR repeats. We divided the individuals of the Human Genome Diversity Panel (HGDP)-CEPH panel into 26 populations according to Barreiro et al.[20] . We used the VNTR locus as a marker to calculate genetic distances between populations. Under the ''outof-Africa'' (OFA) model, all modern humans originated from East African [22] , it implies that the population from East Africa has the highest genetic diversity, and the genetic distance from non-African to East African declines monotonically with the geographical distance away from East Africa. By defining the northeastern Bantu of Kenya as the Human Original region population, we calculated the genetic distance between the other 25 non-African populations and the original population (East African population). Indeed, the VNTR genetic distances between the East Africa and the 25 different populations significantly correlated with their geographical distance to East Africa (R 2 = 0.51, P,0.0001 by linear regression) ( Figure 3 ). The data indicated that the present diversity distribution of the VNTR locus in CLEC4M gene could be explained by human migration in keeping with the OFA model of human settlement history. The patterns of population variation of VNTR in modern humans could be accounted by neutral evolution, that is, the evolution of VNTR in CLEC4M gene was influenced mostly by genetic drift. In this work, by undertaking a comprehensive clonal sequencing study of the internal structure variation within the observed repeats among different populations at the worldwide scale, we gain insights into the evolutionary mechanism underlying the VNTR of CLEC4M gene. The CLEC4M gene plays an important role in innate immunity as pathogen receptor and had been studied as susceptibility gene to infectious and generated conflicting results [11] [12] [13] 15, 16, 18, 19] . As the VNTR is the focus at issue, the study about it is urgent. Understanding of the origin and evolution of the VNTR polymorphism will provide us better insight on whether the VNTR had been a target of natural selection, as an example of the evolution of other immunity related genes. In conclusion, we showed that various VNTR alleles in VNTR locus of CLEC4M gene were present before the time of human dispersion out of Africa. Further analysis showed that the present worldwide diversity profile of this VNTR locus could be resulted from demographic migrating of different tribes, and no evidence was found to support the notion of multiple independent mutation events at this VNTR due to natural selection. Future work based on much more comprehensive sequence information from more species, such as chimpanzee, gibbon, bonobo, could further our understanding of evolution of this gene and the effect of different pathogen pressures across the different species of the primates. ment of all the individuals met the criteria set by the HGDP Ethics Committee. The ethics of informed consent are specifically addressed by the HGDP's ''Model Ethical Protocol for Collecting DNA Samples'', which has been published as [23] . Our present study was performed according to the Declaration of Helsinki. This sample set covered all types of repeats (4-to 9-repeat) in VNTR locus in each continent, based on the data of the CLEC4M neck-region variation in the HGDP-CEPH panel including 1064 individuals from 52 worldwide populations (our unpublished data). The VNTR polymorphism of the neck-region was genotyped as described in Li et al [18] . The genotype was determined by separating the PCR products in 3% agarose gel with ethidium bromide staining. To validate the genotyping results, 10% of the samples were re-genotyped by duplicated genotyping experiments. Clonal sequencing of VNTR in CLEC4M gene was performed by directly sequencing of cloned PCR products. First, the fragment of exon 4 in CLEC4M gene was amplified by the primers, F-CCCTAA GTCAGGAACAATCCGA, R-TCACAGGGGAG-GAAACTGAG. PCR was performed in a 50 ml volume with 50 ng genomic DNA as template, 5 ml PCR 106 buffer, 4 ml dNTP mix (2.5 mM), 2 ml primers (10 pM), 1.25 unit of Taq DNA polymerase (Takara) and 38 ml D.W water. Thermal cycling in a Gene Amp 9700 (Perkin Elmer) thermal cycler was performed at 95uC for 5 min, followed by 40 cycles at 95uC for 20 s, 59uC for 30 s, 72uC for 60 s and extension at 72uC for 5 min. The PCR products were purified on spin columns (Watson BioTechnologies Inc., Shanghai) according to manufacturer's protocol. Then, the purified PCR products were cloned into PMD 18-T Vector (Takara, Japan) and transferred into an ultracompetent cell (Takara, Japan). Then, plasmids carrying a PCR fragment were extracted and sequenced in both directions directly by primers, SF-AGGAACAATCCGAGCAAGACG and SR-AGAGACCA-TCTCAGGCCCAAG, with an ABI 3730 automatic sequencer. For each PCR product, at least 5 clones were chosen at random and sequenced in order to reduce artifactual error leading to single nucleotide variants and artificial recombination due to PCR. The sequencing results were processed by DNASTAR software (DNASTAR) and manual rectification. As the VNTR is composed of a variable number of a basic subunit of 69 base pairs, we analyzed all the sequence variants within each of the subunit. Then, all sequence reads of the 69-bp subunit of VNTR were aligned using the Clustal W program [24] . We only observed 8 different sequence haplotypes (Figure 1 ). According to the sequence variation in the 69-bp fragment, all the subunits could be unique named as one of the 8 different haplotypes. The clonal sequence of the 290 chromosomes of the worldwide population sample then called according to the subunit haplotype (H1 to H8). For example, the common 7-repeat VNTR allele is formed by one H1, three H2, one each of H3, H4, and H5 in the order of H1-H2-H2-H2-H3-H4-H5 ( Figure 2 and Table 1 ). The genotype data of VNTR locus in CLEC4M gene were used to calculate the genetic distance between populations. First, the samples of the Human Genome Diversity Panel (HGDP)-CEPH panel were divided into 26 populations as used in the study of Barreiro et al [20] . Then, the population from northeastern Bantu of Kenya was defined as the Human Original region population. Genetic distances between populations (Fst) (the other 25 non-African populations and the defined original region's population) were estimated using Arlequin package [25] . Correlation analysis between the graphical distance and genetic population distance was carried out using Pearson bivariate correction analysis (SPSS for Windows; 13.0). DC-SIGNR, a DC-SIGN homologue expressed in endothelial cells, binds to human and simian immunodeficiency viruses and activates infection in trans DC-SIGN (dendritic cell-specific ICAM-grabbing nonintegrin) and DC-SIGN-related (DC-SIGNR): friend or foe? C-type lectins DC-SIGN and L-SIGN mediate cellular entry by Ebola virus in cis and in trans Identification of DC-SIGN, a novel dendritic cell-specific ICAM-3 receptor that supports primary immune responses DC-SIGN and L-SIGN are high affinity binding receptors for hepatitis C virus glycoprotein E2 L-SIGN (CD 209L) is a liver-specific capture receptor for hepatitis C virus A dendritic cell-specific intercellular adhesion molecule 3-grabbing nonintegrin (DC-SIGN)-related protein is highly expressed on human liver sinusoidal endothelial cells and promotes HIV-1 infection Novel member of the CD209 (DC-SIGN) gene family in primates Extended neck regions stabilize tetramers of the receptors DC-SIGN and DC-SIGNR DC-SIGN; a related gene, DC-SIGNR; and CD23 form a cluster on 19p13 DC-SIGNR neck-region polymorphisms and HIV-1 susceptibility: From population stratification to a possible advantage of the 7/5 heterozygous genotype Homozygous L-SIGN (CLEC4M) plays a protective role in SARS coronavirus infection The tandem-repeat polymorphism of the DC-SIGNR gene does not affect the susceptibility to HIV infection and the progression to AIDS Repeat-region polymorphisms in the gene for the dendritic cell-specific intercellular adhesion molecule-3-grabbing nonintegrin-related molecule: effects on HIV-1 susceptibility The tandem-repeat polymorphism of the DC-SIGNR gene in HCV infection Length variation of DC-SIGN and L-SIGN neck-region has no impact on tuberculosis susceptibility DC-SIGN and DC-SIGNR genetic diversity among different ethnic populations: potential implications for pathogen recognition and disease susceptibility Polymorphisms in the C-type lectin genes cluster in chromosome 19 and predisposition to severe acute respiratory syndrome coronavirus (SARS-CoV) infection Lack of support for an association between CLEC4M homozygosity and protection against SARS coronavirus infection The heritage of pathogen pressures and ancient demography in the human innateimmunity CD209/CD209L region A human genome diversity cell line panel Genetic and fossil evidence for the origin of modern humans Proposed Model Ethical Protocol for Collecting DNA Samples CLUSTAL W: improving the sensitivity of progressive multiple sequence alignment through sequence weighting, position-specific gap penalties and weight matrix choice Arlequin (version 3.0): an integrated software package for population genetics data analysis We are grateful to all the participants in this research. We also would like to acknowledge Shi-Fang Wu and Chun-Ling Zhu for their help in experiments.