虹鳟Scarb1基因克隆、生物信息学及组织表达分析

清道夫受体B类成员1(scavenger receptor class B member 1,Scarb1)作为细胞表面的膜受体蛋白,在动物体色形成过程中发挥重要作用。为了解Scarb1基因在虹鳟(Oncorhynchus mykiss)体色形成中的作用,通过RACE技术克隆虹鳟Scarb1基因的cDNA全长,并运用生物信息学方法分析该基因及其序列结构特征,同时使用实时定量PCR(qRT-PCR)检测Scarb1基因在虹鳟、金鳟及其杂交F_(1)代不同发育阶段和不同组织中的表达情况。结果显示,Scarb1基因cDNA序列全长为2032 bp,开放阅读框1479 bp,编码492个氨基酸,预测分子质量为55.59 ku,且存在保守的CD36结构域和2个跨膜区。序列同源性分析显示,虹鳟与其他硬骨鱼类的氨基酸序列相似度为71.69%~98.58%;进化分析发现虹鳟与大马哈鱼亲缘关系最近,与哺乳动物和两栖动物亲缘关系最远。qRT-PCR检测结果表明,在虹鳟与金鳟胚胎期及出膜后各发育阶段中Scarb1基因均有不同程度表达,且表现为受精期至桑葚期的表达显著高于其他时期(P<0.05),对虹鳟与金鳟同一时期的差异分析发现该基因在胚胎期及7 dph(days post hatch)、1 M(month post hatch)、2 M和3 M时期中表达存在显著差异(P<0.01)。Scarb1基因在虹鳟与金鳟背部皮肤和背部肌肉等色素沉着性组织中表达量较高,其中在金鳟背部皮肤的表达量显著高于虹鳟(P<0.01)。此外,Scarb1基因在杂交F_(1)代不同发育时期中的表达规律与双亲一致;在不同组织中,该基因在杂交F_(1)代背部皮肤中的表达量介于双亲之间。研究结果表明,Scarb1基因与虹鳟体色形成有着密切关系,且可能在金鳟黄色体色形成过程中发挥重要作用。

Identification and effective regulation of scarb1 gene involved in pigmentation change in autotetraploid Carassius auratus

The autotetraploid Carassius auratus(4nRR,4n=200,RRRR)is derived from whole-genome duplication of Carassius auratus red var.(RCC,2n=100,RR).In the current study,we demonstrated that chromatophores and pigment changes directly caused the coloration and variation of 4nRR skin(red in RCC,brownish-yellow in4nRR).To further explore the molecular mechanisms underlying coloration formation and variation in 4nRR,we performed transcriptome profiling and molecular functional verification in RCC and 4nRR.Results revealed that scarb1,associated with carotenoid metabolism,underwent significant down-regulation in 4nRR.Efficient editing of this candidate pigment gene provided clear evidence of its significant role in RCC coloration.Subsequently,we identified four divergent scarb1 homeologs in 4nRR:two original scarb1 homeologs from RCC and two duplicated ones.Notably,three of these homeologs possessed two highly conserved alleles,exhibiting biased and allelespecific expression in the skin.Remarkably,after precise editing of both the original and duplicated scarb1homeologs and/or alleles,4nRR individuals,whether singly or multiply mutated,displayed a transition from brownishyellow skin to a cyan-gray phenotype.Concurrently,the proportional areas of the cyan-gray regions displayed a gene-dose correlation.These findings illustrate the subfunctionalization of duplicated scarb1,with all scarb1genes synergistically and equally contributing to the pigmentation of 4nRR.This is the first report concerning the functional differentiation of duplicated homeologs in an autopolyploidfish,substantiallyenrichingour understanding of coloration formation and change within this group of organisms.

中华绒螯蟹Scarb1基因功能及其与生长性状的关联分析

为研究B类Ⅰ型清道夫受体(SCARB1/SR-BI)在中华绒螯蟹代谢、生长以及免疫等生物学过程中的分子功能,实验对中华绒螯蟹Scarb1的克隆及时空表达进行了分析,观察了RNA干扰该基因后的相关组织结构和类胡萝卜素含量变化,筛选了该基因的SNP标记并与生长相关性状进行关联分析。结果显示,中华绒螯蟹的Scarb1由2个外显子和1个内含子组成,开放阅读框为2415 bp,编码805个氨基酸;系统进化分析显示中华绒螯蟹与三疣梭子蟹的氨基酸同源性高达80.51%,具有较高的物种间保守性。该基因在不同蜕壳时期的肝胰腺、肠道、血淋巴细胞、心脏、鳃和肌肉组织中均有表达,但在肝胰腺、肠道和血淋巴细胞中的表达量相对较高。RNA干扰Scarb1后,组织切片观察发现肝胰腺的肝小管管腔模糊并产生了部分空泡化结构,肠道内膜的肌肉层和黏膜下层处出现显著空洞现象;肝胰腺的颜色由黄色变成灰白色,其中的类胡萝卜素含量显著下降。在该基因的第一外显子筛选到1个SNP位点(C432T)与蜕壳后体重和壳长增长率存在显著相关性。本研究结果为Scarb1在中华绒螯蟹的遗传研究和育种应用提供参考。

瓯江彩鲤Scarb 1基因敲除自交子一代的体色相关性状观察

为了解瓯江彩鲤基因敲除体在自交繁育过程中的体色遗传和变异情况,对野生型和敲除了Scarb 1基因的敲除型自繁F_(1)全红、粉玉体色瓯江彩鲤个体的鳞片色素细胞进行了观察比较,并测定了其体内的类胡萝卜素含量。结果显示:野生型全红瓯江彩鲤的鳞片含有黄色素细胞、红色素细胞和虹彩细胞,而敲除型全红瓯江彩鲤的鳞片上只有黄色素细胞和虹彩细胞,没有红色素细胞;野生型和敲除型粉玉瓯江彩鲤的鳞片色素细胞均为虹彩细胞,没有黄色素和红色素细胞;野生型全红瓯江彩鲤的肠道、血浆、肌肉和皮肤中的类胡萝卜素含量均显著高于敲除型全红个体(P<0.05);野生型粉玉瓯江彩鲤的肠道、肌肉和鳍条中的类胡萝卜素含量也显著高于敲除型粉玉个体(P<0.05)。研究结果表明,敲除Scarb 1基因影响了瓯江彩鲤体表红色素细胞的生成,该基因在瓯江彩鲤红、白体色调控中发挥作用。

CA16感染树鼩肺成纤维细胞模型的建立及其受体SCARB2的表达

目的 探讨建立CA16感染树鼩肺成纤维细胞(tree shrew lung fibroblasts,TSLF)实验模型的可行性。方法 用肠道病毒CA16感染TSLF,以人肺成纤维细胞(KMB-17)作对照,镜下观察细胞病变情况,间接免疫荧光实验观察病毒蛋白和感染相关受体SCARB2蛋白的表达情况,探针法实时荧光定量PCR检测病毒载量,以β-Actin作内参染料法实时荧光定量PCR检测受体SCARB2基因的相对表达量,结合基因序列比对,分析其与感染的相关性。结果 CA16感染TSLF,可引起明显的细胞病变,免疫荧光实验可见病毒和受体SCARB2蛋白,以100TCID50/10^5 cells的比例感染TSLF可在48 h左右病毒载量达到最高,SCARB2基因有与感染相关的高表达,而其基因序列也与人有较高同源性。结论 CA16可感染TSLF,树鼩SCARB2可参与感染。

人SCARB2蛋白提高人肠道病毒71型对转基因小鼠的感染力

目的细胞实验证实人清道夫受体B2(hSCARB2)是人类EV71的受体,本研究拟通过建立人SCARB2转基因小鼠,建立感染能力更高的小鼠模型。方法构建CMV启动子的SCARB2转基因表达载体,通过显微注射法建立C57BL/6J背景的人SCARB2转基因小鼠,PCR筛选阳性首建鼠。通过Western Blot和免疫组化检测目的蛋白在各组织中的表达。EV71感染转基因小鼠后,通过实时荧光定量PCR和免疫组化检测目的蛋白表达对病毒感染的促进效果。结果人SCARB2蛋白主要在转基因小鼠的骨骼肌和脑组织中表达,与野生型小鼠相比,转基因小鼠组织中的病毒载量显著提高4到5倍。结论人SCARB2的体内表达可促进EV71对转基因小鼠的感染,该蛋白在体内具有EV71受体功能。

SCARB1在肾癌中表达上调并与其不良预后相关

目的:探讨调控脂肪代谢的清道夫受体B1基因(SCARB1)与肾癌的关系及其潜在的生物学作用。方法:比较TCGA肿瘤数据库内正常肾脏和肾癌组织内SCARB1 mRNA表达的差异,采用免疫组织化学检测正常肾脏和肾癌组织内SCARB1蛋白的表达情况;分析SCARB1基因拷贝数与甲基化情况,探究SCARB1在肾癌内表达异常的原因;采用Kaplan-Meier生存分析SCARB1与肾癌患者总体生存的关系;采用油红染色检测SCARB1低表达和高表达肾癌组织内脂肪的含量;最后分析SCARB1与脂肪代谢关键基因SCD表达的相关性。结果:肾癌组织内SCARB1 mRNA及蛋白表达水平明显高于正常肾脏组织;DNA拷贝数分析肾癌组织内SCARB1基因存在扩增现象,且SCARB1基因的甲基化与其mRNA的表达水平呈现明显负相关。生存分析提示SCARB1高表达的肾癌患者总体生存率明显减低。此外,SCARB1高表达的肾癌组织内脂肪含量增加,且与脂肪调控基因SCD1的表达水平呈显著正相关。结论:SCARB1在肾癌中表达上调并与其不良预后相关;SCARB1可能在肾癌的脂肪合成过程中发挥重要作用。

人体多组织器官EV 71病毒受体SCARB 2和PSGL-1的分布特点

目的探讨人体多组织器官中EV71病毒受体SCARB2和PSGL-1的分布特点及其意义。方法应用免疫组织化学法检测中枢神经、呼吸道、肠道、肝脏、脾脏、心脏组织EV71病毒受体SCARB2和PSGL-1的表达。结果 SCARB2在中枢神经的大脑、小脑、脑干,呼吸道的喉部、气管、支气管、细支气管、肺泡细胞、巨噬细胞以及肠道组织中呈阳性分布,肝脏呈弱阳性或阴性,脾脏、心脏则为阴性,SCARB2受体在中枢神经、呼吸道和肠道的分布明显高于肝脏、脾脏、心脏(P<0.05)。PSGL-1在中枢神经的大脑、小脑、脑干,呼吸道的喉部呈阳性分布,呼吸道的气管、支气管、肠道呈少量阳性分布,而肺泡细胞阴性,肝脏、脾脏、心脏为阴性或仅极少量表达阳性。PSGL-1受体在中枢神经系统的分布明显高于呼吸道、肠道、肝脏、脾脏、心脏(P<0.05),PSGL-1受体在呼吸道、肠道的分布明显高于肝脏、脾脏、心脏(P<0.05)。结论在中枢神经、呼吸道和肠道表达的EV71病毒受体SCARB2和/或PSGL-1,提示上述组织器官是EV71感染的主要部位。

SCARB2基因突变致动作性肌阵挛―肾衰综合征

背景动作性肌阵挛―肾衰综合征(AMRF)是进行性肌阵挛性癫痫(PME)的一种类型,是一种常染色体隐性遗传性疾病,与SCARB2基因的突变相关。目的报道SCARB2基因突变相关性AMRF家系的1个病例,并总结目前所有文献报道的AMRF患者的临床表型和遗传学特征,以提高对该病的认识。方法回顾AMRF患者的临床资料,采用全外显子组基因靶向二代测序对AMRF家系的1个病例进行基因检测。结合文献报道,对28例(包含本例)AMRF病例资料进行总结分析。结果AMRF患者主要临床特征为动作性肌阵挛、全身性强直阵挛性癫痫、共济失调、无认知功能障碍、伴或不伴肾功能障碍。先证者携带SCARB2基因纯合移码突变(c.350_351delAT,p.Y117Cfs*3,NM_005506.3)。先证者未患病的母亲及姐姐携带该位点的单杂合突变。国际上目前报道的28例(包括本例)SCARB2基因突变相关性AMRF中共发现22种不同的突变位点,均以常染色体隐性遗传方式发病。结论该研究在与SCARB2基因突变相关的AMRF患者中发现了1个未见报道过的新的移码突变位点。结合文献复习,可推测当突变位点位于更靠近5端和更重要的功能域时,对蛋白产物功能的影响会更大。

手足口病伴神经病变患儿血管内皮细胞生长因子、血管细胞黏附分子-1、SCARB2水平变化

目的观察手足口病伴神经病变患儿的血管内皮生长因子(VEGF)、血管细胞黏附分子-1(VCAM-1)、SCARB2水平变化并分析其临床意义。方法2017年3月至2018年12月该院收治的手足口病患儿120例,根据其是否伴神经病变分为对照组和观察组。观察两组血清VEGF、VCAM-1、SCARB2,可溶性人白细胞抗原G(sHLA-G)、IL-6、IL-10,WBC、中性粒细胞(N)和淋巴细胞(L)水平变化。结果观察组血清VEGF、VCAM-1水平及SCARB2阳性率明显高于对照组,sHLA-G、IL-6、IL-10及WBC、N、L浓度均高于对照组。结论手足口病伴神经病变患儿的VEGF、VCAM-1、SCARB2水平较高,且IL-6等细胞因子水平及血白细胞浓度也随之升高,可考虑作为临床重点监测的指标。

H19 recruited N^(6)-methyladenosine(m^(6)A)reader YTHDF1 to promote SCARB1 translation and facilitate angiogenesis in gastric cancer

Background:Angiogenesis is described as a complex process in which new microvessels sprout from endothelial cells of existing vasculature.This study aimed to determine whether long non-coding RNA(lncRNA)H19 induced the angiogenesis of gastric cancer(GC)and its possible mechanism.Methods:Gene expression level was determined by quantitative real-time polymerase chain reaction and western blotting.Cell counting kit-8,transwell,5-Ethynyl-2′-deoxyuridine(EdU),colony formation assay,and human umbilical vein endothelial cells(HUVECs)angiogenesis assay as well as Matrigel plug assay were conducted to study the proliferation,migration,and angiogenesis of GC in vitro and in vivo.The binding protein of H19 was found by RNA pull-down and RNA Immunoprecipitation(RIP).High-throughput sequencing was performed and next Gene Ontology(GO)as well as Kyoto Encyclopedia of Genes and Genomes(KEGG)analysis was conducted to analyze the genes that are under H19 regulation.Methylated RIP(me-RIP)assay was used to investigate the sites and abundance among target mRNA.The transcription factor acted as upstream of H19 was determined through chromatin immunoprecipitation(ChIP)and luciferase assay.Results:In this study,we found that hypoxia-induced factor(HIF)-1a could bind to the promoter region of H19,leading to H19 overexpression.High expression of H19 was correlated with angiogenesis in GC,and H19 knocking down could inhibit cell proliferation,migration and angiogenesis.Mechanistically,the oncogenic role of H19 was achieved by binding with the N^(6)-methyladenosine(m^(6)A)reader YTH domain-containing family protein 1(YTHDF1),which could recognize the m^(6)A site on the 3′-untransated regions(3′-UTR)of scavenger receptor class B member 1(SCARB1)mRNA,resulting in over-translation of SCARB1 and thus promoting the proliferation,migration,and angiogenesis of GC cells.Conclusion:HIF-1a induced overexpression of H19 via binding with the promoter of H19,and H19 promoted GC cells proliferation,migration and angiogenesis through YTHDF1/SCARB1,which might be a beneficial target for antiangiogenic therapy for GC.

miR-125a-5p靶向Scarb1基因对缺氧/复氧心肌细胞损伤的影响及其机制研究

目的探讨miR-125a-5p靶向调控清道夫受体B1(Scarb1)基因对缺氧/复氧大鼠心肌细胞损伤的影响及作用机制。方法将体外培养的H9c2大鼠心肌细胞随机分为空白对照组、缺氧/复氧组、转染对照组和miR-125a-5p转染组。检测各组miR-125a-5p的表达量、心肌细胞的活力、凋亡率、ATP含量以及Scarb1、Cyt C、Bax、Bcl-2及NF-κB信号通路相关蛋白的表达情况。利用Targetscan软件预测miR-125a-5p的靶基因,用双荧光素酶报告基因实验验证miR-125a-5p和Scarb1的靶向关系。结果与空白对照组相比,缺氧/复氧组心肌细胞miR-125a-5p、Bax、Cyt C的表达和凋亡率明显升高(P<0.05),细胞活力、Scarb1、Bcl-2的表达及ATP含量明显降低(P<0.05)。与转染对照组相比,miR-125a-5p转染组的情况与上述变化相反。双荧光素酶报告基因实验证实Scarb1为miR-125a-5p的靶基因。缺氧/复氧能够促进心肌细胞中NF-κB p65、c-Myc和Cyclin D1蛋白的表达,而下调miR-125a-5p的表达则能够抑制上述蛋白的表达。结论缺氧/复氧能够诱导心肌细胞中miR-125a-5p的表达,抑制miR-125a-5p则能够通过上调Scarb1的表达对缺氧/复氧心肌细胞起保护作用,其机制可能与抑制NF-κB信号通路的活化有关。

清道夫受体B1基因(SCARB1)多态性与心血管疾病发病风险相关性的Meta分析

目的系统评价清道夫受体B1基因(SCARB1)变异与心血管疾病(CVD)发病风险的相关性。方法计算机检索PubMed、Web of Science、CNKI、WanFang Data和VIP数据库,检索时限均从建库截至2017年12月31日。由两位研究者独立筛选文献、提取资料和评价纳入研究的偏倚风险后,采用Stata 12.0软件进行Meta分析。结果共纳入12个研究,报告了SCARB1基因rs5888 C/T多态性、rs4238001 G/A多态性和rs10846744G/C多态性与心血管疾病易感性的相关性。Meta分析结果显示,rs10846744 G/C多态性与心血管疾病发病风险相关[G vs. C:OR=1.30,95%CI(1.11,1.52),P=0.001],但rs5888 C/T多态性[C vs. T:OR=0.97,95%CI(0.86,1.09),P=0.627]和rs4238001 G/A多态性[G vs. A:OR=0.87,95%CI(0.64,1.17),P=0.344]与心血管疾病发病风险不相关。亚组分析结果显示:rs5888 C/T多态性与非亚洲人群CVD的发病风险相关[C vs. T:OR=0.82,95%CI(0.68,0.99),P=0.040]。结论 SCARB1 rs10846744 G/C多态性与CVD发病风险相关。但受纳入研究的数量和质量的限制,上述结论尚待开展更多高质量研究予以验证。

Molecular mechanism of SCARB2-mediatec attachment and uncoating of EV71

Unlike the well-established picture for the entry of enveloped viruses, the mechanism of cellular entry of non-enveloped eukaryotic viruses remains largely mysterious. Picornaviruses are representative models for such viruses, and initiate this entry process by their functional receptors. Here we present the structural and functional studies of SCARB2, a functional receptor of the important human enterovirus 71 （EV71）. SCARB2 is responsible for attachment as well as uncoating of EV71. Differences in the structures of SCARB2 under neutral and acidic conditions reveal that SCARB2 undergoes a pivotal pH-dependent conformational change which opens a lipid-transfer tunnel to mediate the expulsion of a hydrophobic pocket factor from the virion, a pre-requisite for uncoating. We have also identified the key residues essential for attachment to SCARB2, identifying the canyon region of EV71 as mediating the receptor interaction. Together these results provide a clear understanding of cellular attachment and initiation of uncoating for enteroviruses.

The binding of a monoclonal antibody to the apical region of SCARB2 blocks EV71 infection

Entero virus 71 （EV71） causes hand, foot, and mouth disease （HFMD） and occasionally leads to severe neurological complications and even death. Scavenger receptor class B member 2 （SCARB2） is a functional receptor for EV71, that mediates viral attachment, internalization, and uncoating. However, the exact binding site of EV71 on SCARB2 is unknown. In this study, we generated a monoclonal antibody （mAb） that binds to human but not mouse SCARB2. It is named JL2, and it can effectively inhibit EV71 infection of target cells. Using a set of chimeras of human and mouse SCARB2, we identified that the region containing residues 77-113 of human SCARB2 contributes significantly to JL2 binding. The structure of the SCARB2-JL2 complex revealed that JL2 binds to the apical region of SCARB2 involving a-helices 2, 5, and 14. Our results provide new insights into the potential binding sites for EV71 on SCARB2 and the molecular mechanism of EV71 entry.

Identification of a Novel Homozygous Splice-Site Mutation in SCARB2 that Causes Progressive Myoclonus Epilepsy with or without Renal Failure

Background： Progressive myoclonus epilepsies （PMEs） conaprise a group of rare genetic disorders characterized by action rnyoclonus, epileptic seizures, and ataxia with progressive neurologic decline. Due to clinical and genetic heterogeneity of PMEs, it is difficult to decide which genes are affected. The aim of this study was to report an action myoclonus with or without renal failure syndrome （EPM4） fhmily and summarize the clinical and genetic characteristics of all reported EPM4 patients. Meihods： In the present study, targeted next-generation sequencing （NGS） was applied to screen causative genes in a Chinese PME family. The candidaie variant was further confirmed by cosegregation analysis and further functional analysis, including the reverse transcription polymerase chain reaction and Western blot of the proband＇s muscle. Moreovel, literature data on the clinical and mutational features of all reported EPM4 patients were reviewed. Results： The gene analysis revealed a novel homozygous splicing mutation （c.995-1G〉A） of the SCARB2 gene in two brothers. Further functional analysis revealed that this mutation led to loss function of the SCARB2 protein. The classification of the candidate variant, according to the American College of Medical Genetics and Genomics standards and guidelines and functional analysis, was pathogenic. Therefore, these two brothers were finally diagnostically confirmed as EPM4. Conclusions： These present results suggest the potential for targeted NGS to conduct a more rapid and precise diagnosis for PME patients. A literature review revealed that mutations in the different functional domains of SCARB2 appear to be associated with the phenotype of EPM4.

SCARB2基因突变致动作性肌阵挛癫痫肾衰竭综合征1例

文中报道1例动作性肌阵挛癫痫-肾衰竭综合征(AMRF)患者的临床、电生理、肾脏病理及基因突变特点。患者为青年男性,16岁以癫痫起病,逐渐出现震颤、共济失调、肌阵挛发作。颅脑磁共振成像未见明显异常。神经电生理表现为四肢对称性、多发性感觉神经和运动神经传导速度减慢,以神经易嵌压部位为著。肾脏病理表现为局灶性节段性肾小球硬化。基因检测发现该患者SCARB2基因存在新的复合杂合突变:c.534_537delinsCT(chr4:7710074)及c.358G>T(chr4:7710217),经过家系验证2处杂合突变分别来自患者父母。AMRF是青少年癫痫中的罕见类型,本病早期表现为肌阵挛或肾功能异常,临床异质性较大,容易误诊漏诊。其最终确诊依赖基因检测。

中国山西汉族人群rs5888及rs1207568位点单核苷酸多态性与脑梗死合并糖尿病易感性的关系

目的研究中国山西汉族人群SCARB1基因rs5888位点及Klotho基因rs1207568位点单核苷酸多态性与脑梗死合并糖尿病易感性的关系,为脑梗死发病分子机制的进一步研究提供科学依据。方法首先通过生物信息学的手段分析SCARB1和Klotho基因及蛋白质组学信息。选择49例被确诊脑梗死合并糖尿病的患者、52例被确诊为患有脑梗死的患者及39例被确诊患有糖尿病的患者为研究对象,并选择33例无脑梗死和糖尿病的受试者为对照组。经测序分析确定各组受试者的SCARB1基因rs5888位点及Klotho基因rs1207568位点的基因型,并对其结果进行统计分析。结果SCARB1及Klotho基因的生物信息学预测结果和文献报道的蛋白性质一致。测序结果表明SCARB1基因及Klotho基因分别存在rs5888及rs1207568位点上的基因多态性。Klotho rs1207568不同基因型间临床参数比较,除脑梗死合并糖尿病组尿酸(UA)和单纯性糖尿病组甘油三酯(TG)差异有统计学意义(P<0.05)外,其他临床参数的差异均没有统计学意义(P>0.05)。SCARB1 rs5888 CC和CT/TT基因型病例的临床参数间比较,只有单纯性糖尿病组两种基因型的病例之间活化部分凝血活酶时间(APTT)差异有统计学意义(P<0.05),其他临床参数的差异均没有统计学意义(P>0.05)。脑梗死合并糖尿病患者组SCARB1 rs5888的CT/TT频率明显高于对照组,但CC频率低于对照组(P<0.05)。各组间在Klotho rs1207568中的CT/TT和CC频率差异无统计学意义(P>0.05)。结论SCARB1基因rs5888及Klotho基因rs1207568单核苷酸多态性可能是评估脑梗死合并糖尿病易感性的重要分子标志物。

基于类胡萝卜素着色的鸟类羽色多样性形成机制

人们对动物体色的研究由来已久。作为一类让生物呈现出多变色彩的重要色素,类胡萝卜素可以在鸟类的羽毛、鸟喙和皮肤等体表组织中沉积,产生红、橙、黄、粉、紫等颜色。类胡萝卜素不能在鸟类体内合成,需从食物中摄取,进而在体内完成吸收、运输、代谢和沉积等一系列过程,才能用于羽毛着色。与类胡萝卜素着色相关的生理及遗传调控机制一直备受关注,BCO2、SCARB1和CYP2J19等影响类胡萝卜素在鸟类羽毛中着色的关键基因,推动了对羽色遗传调控机制的深入认识。本文介绍了鸟类可利用类胡萝卜素的主要类型和基本特征,综述了类胡萝卜素着色相关的生理过程以及调控基因研究的最新进展,旨在增加对鸟类羽毛中类胡萝卜素着色过程和相关遗传机制的理解。