Article(id=1211258400625791116, tenantId=1146029695717560320, journalId=1149651085930835976, issueId=1211258399447191684, articleNumber=null, orderNo=null, doi=10.12284/hyxb2023004, pmid=null, cstr=null, oa=null, hot=null, price=null, onlineType=0, articleFormat=0, articleType=null, articleTypeStr=research-article, receivedDate=1648137600000, receivedDateStr=2022-03-25, revisedDate=1656000000000, revisedDateStr=2022-06-24, acceptedDate=null, acceptedDateStr=null, onlineDate=1766716106802, onlineDateStr=2025-12-26, pubDate=1672502400000, pubDateStr=2023-01-01, doiRegisterDate=null, doiRegisterDateStr=null, onlineIssueDate=1766716106802, onlineIssueDateStr=2025-12-26, onlineJustAcceptDate=null, onlineJustAcceptDateStr=null, onlineFirstDate=null, onlineFirstDateStr=null, sourceXml=null, magXml=null, createTime=1766716106802, creator=13701087609, updateTime=1766716106802, updator=13701087609, issue=Issue{id=1211258399447191684, tenantId=1146029695717560320, journalId=1149651085930835976, year='2023', volume='45', issue='1', pageStart='1', pageEnd='70', issueExtLink='null', onlineDate='null', pubDate='null', beforeIssueId=null, nextIssueId=null, price=null, status=1, issueComplete=1, articleOrder=1, issueType=-1, specialIssue=null, createTime=1766716106520, creator=13701087609, updateTime=1766734463188, updator=13701087609, preIssue=null, nextIssue=null, ext={EN=IssueExt(id=1211335392964506397, tenantId=1146029695717560320, journalId=1149651085930835976, issueId=1211258399447191684, language=EN, specialIssueTitle=, coverIllustrator=null, specialIssueEditor=, specialIssueAbout=), CN=IssueExt(id=1211335392964506398, tenantId=1146029695717560320, journalId=1149651085930835976, issueId=1211258399447191684, language=CN, specialIssueTitle=, coverIllustrator=null, specialIssueEditor=, specialIssueAbout=)}, issueFiles=null}, startPage=62, endPage=70, ext={EN=ArticleExt(id=1211258400835506321, articleId=1211258400625791116, tenantId=1146029695717560320, journalId=1149651085930835976, language=EN, title=Effects of sulfide stress on blood ${{\bf {SO}} _4^{2-}} $ concentration and SULT1B1-12 gene expression in Sinonovacula constricta, columnId=1194652705852465724, journalTitle=Haiyang Xuebao, columnName=Article, runingTitle=null, highlight=null, articleAbstract=

As a typical dwelled tidal shellfish, Sinonovacula constricta is often exposed to sulfide-rich environment and shows strong sulfide tolerance. The cytosolic sulfotransferase 1B1 (SULT1B1) is located at downstream of the sulfur metabolism pathway, while it is a key enzyme catalyzing the sulfation reaction and plays an important role in the biotransformation of endogenous substances such as thyroid hormones (THs). In order to study the role of ScSULT1B1-12 in sulfur resistance, the sequence characteristics were analyzed by bioinformatics method. Combined with the changes of blood ${\rm {SO}} _4^{2-} $ concentration, the spatial expression and temporal expression profiles during 72 h sulfide stress (50 μmol/L, 150 μmol/L, 300 μmol/L) were studied. The full-length cDNA of ScSULT1B1-12 gene was 1 100 bp, containing an open reading frame of 897 bp, and encoding 298 amino acids. Sequence analysis showed that ScSULT1B1-12 contains four catalytic active sites (56K, 104N, 106H, and 134A), one PAPS binding domain (YPKSGTXW) at N terminal, and one PAPS binding and dimerization domain (RKGXXGDWKNXFTVXXE) at C terminal, indicating that it was structurally able to catalyze the sulfation reaction. Spatial expression showed that ScSULT1B1-12 was highly expressed in gills, followed by the adductor muscle and hepatopancreas. Blood ${\rm {SO}} _4^{2-} $ concentration decreased, and the expression patterns of ScSULT1B1-12 also declined with fluctuation after sulfide stress, indicating that sulfate can be further transformed to sulfated donors, and ScSULT1B1-12-mediated sulfation may be inhibited to keep THs at a certain level in S. constricta, in order to strengthen the metabolic and immune functions, and make the organism adapt the adverse environment of high sulfide.

, correspAuthors=Caifang Chen, authorNote=null, correspAuthorsNote=null, copyrightStatement=Copyright © 2023 Pratacultural Science. All rights reserved., copyrightOwner=null, extLink=null, articleAbsUrl=null, sourceXml=null, magXml=null, pdfUrl=null, pdf=null, pdfFileSize=null, pdfExtLink=null, richHtmlUrl=null, mobilePdfUrl=null, reviewReport=null, pdfFirstPage=null, abstractGraph=null, abstractGraphContent=null, abstractVideo=null, citation=null, cebUrl=null, magXmlContent=null, mapNumber=null, authorCompany=null, fund=null, authors=null, authorsList=Huimiao Sun, Weiliang Shen, Caifang Chen, Zhihua Lin, Qingxi Han), CN=ArticleExt(id=1211258402035077315, articleId=1211258400625791116, tenantId=1146029695717560320, journalId=1149651085930835976, language=CN, title=硫化物胁迫对缢蛏血液${\rm {SO}} _4^{2-}$浓度及SULT1B1-12基因表达的影响, columnId=1149698756456657529, journalTitle=海洋学报, columnName=论文, runingTitle=null, highlight=null, articleAbstract=

作为典型的埋栖型滩涂贝类,缢蛏(Sinonovacula constricta)常暴露在富含硫化物的环境中,并表现出较强的硫化物耐受能力。胞质磺基转移酶1B1(SULT1B1)位于硫代谢途径下游,是催化磺化反应的关键酶,在甲状腺激素(THs)等内源性物质的生物转化过程中发挥重要作用。为研究ScSULT1B1-12基因在缢蛏耐硫中的作用,本研究采用生物信息学方法分析了其序列特征,并结合血液中${\rm {SO}} _4^{2-} $浓度变化,开展其组织表达及不同浓度(50 μmol/L、150 μmol/L、300 μmol/L)硫化物胁迫72 h后的表达特征研究。结果表明,ScSULT1B1-12基因全长cDNA为1 100 bp,含有 897 bp的开放阅读框,编码298个氨基酸。序列分析表明,ScSULT1B1-12含有4个催化活性位点(56K、104N、106H和134A)、1个N端的PAPS结合域(YPKSGTXW)、1个C端的PAPS结合和二聚化域(RKGXXGDWKNXFTVXXE),表明其在结构上具有催化磺化反应的能力。组织分布表明,ScSULT1B1-12基因在鳃中高表达,其次为闭壳肌和肝胰腺。硫化物胁迫后缢蛏血液中${\rm {SO}} _4^{2-} $浓度呈下降趋势,ScSULT1B1-12基因的表达模式也在波动中呈下降趋势,表明硫酸盐可进一步被活化生成磺化反应的供体,而ScSULT1B1-12介导的磺化反应受抑制后可使缢蛏体内THs保持在一定水平,以加强其代谢机能和免疫功能,使机体适应高硫化物的不良环境。

, correspAuthors=陈彩芳, authorNote=null, correspAuthorsNote=
*陈彩芳,女,博士,副教授,硕士生导师,主要从事海洋生物环境适应性研究。E-mail:
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孙慧妙(1996-),女,浙江省衢州市人,研究方向为滩涂贝类环境适应机制。E-mail:

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Journal of Applied Ichthyology, 2003, 19(2): 118−122., articleTitle=null, refAbstract=null), Reference(id=1215295133482926266, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, doi=null, pmid=null, pmcid=null, year=null, volume=null, issue=null, pageStart=null, pageEnd=null, url=null, language=null, rfNumber=36, rfOrder=42, authorNames=null, journalName=null, refType=null, unstructuredReference=陈勇, 华雪铭, 周洪琪, 等. 壳聚糖和益生菌对异育银鲫非特异免疫功能及血清甲状腺激素、皮质醇水平的影响[J]. 水产学报, 2010, 34(5): 711−718., articleTitle=null, refAbstract=null), Reference(id=1215295133579395262, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, doi=null, pmid=null, pmcid=null, year=null, volume=null, issue=null, pageStart=null, pageEnd=null, url=null, language=null, rfNumber=36, rfOrder=43, authorNames=null, journalName=null, refType=null, unstructuredReference=Chen Yong, Hua Xueming, Zhou Hongqi, et al. 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Journal of Fisheries of China, 2010, 34(5): 711−718., articleTitle=null, refAbstract=null), Reference(id=1215295133642309826, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, doi=null, pmid=null, pmcid=null, year=null, volume=null, issue=null, pageStart=null, pageEnd=null, url=null, language=null, rfNumber=37, rfOrder=44, authorNames=null, journalName=null, refType=null, unstructuredReference=边原, 李刚, 杨勇, 等. 甲状腺激素在免疫应答方面的研究进展[J]. 实用药物与临床, 2015, 18(2): 219−222., articleTitle=null, refAbstract=null), Reference(id=1215295133705224389, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, doi=null, pmid=null, pmcid=null, year=null, volume=null, issue=null, pageStart=null, pageEnd=null, url=null, language=null, rfNumber=37, rfOrder=45, authorNames=null, journalName=null, refType=null, unstructuredReference=Bian Yuan, Li Gang, Yang Yong, et al. Research progress of thyroid hormone upon immune response[J]. Practical Pharmacy and Clinical Remedies, 2015, 18(2): 219−222., articleTitle=null, refAbstract=null)], funds=[Fund(id=1215295129993265227, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, awardId=null, language=CN, fundingSource=浙江省公益技术应用研究项目(LGN22C190025);国家重点研发计划“蓝色粮仓”科技创新课题(2018YFD0901405,2020YFD0900802);财政部和农业农村部:国家现代农业产业技术体系项目(CARS-49);浙江省科技重点研发计划(2019C02054,2021C02069-7)。, fundOrder=null, country=null)], companyList=[AuthorCompany(id=1215295125689910156, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, xref=1, ext=[AuthorCompanyExt(id=1215295125698298765, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, companyId=1215295125689910156, language=CN, country=null, province=null, city=null, postcode=null, companyName=null, departmentName=null, remark=1 浙江万里学院 生物与环境学院 浙江省水产种质资源高效利用技术研究重点实验室,浙江 宁波 315100)]), AuthorCompany(id=1215295125769601938, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, xref=1, ext=[AuthorCompanyExt(id=1215295125777990546, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, companyId=1215295125769601938, language=EN, country=null, province=null, city=null, postcode=null, companyName=null, departmentName=null, remark=1Zhejiang Key Laboratory of Aquatic Germplasm Resources, College of Biological and Environmental Sciences, Zhejiang Wanli University, Ningbo 315100, China)]), AuthorCompany(id=1215295125845099414, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, xref=2, ext=[AuthorCompanyExt(id=1215295125853488023, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, companyId=1215295125845099414, language=CN, country=null, province=null, city=null, postcode=null, companyName=null, departmentName=null, remark=2 宁波大学 海洋学院,浙江 宁波 315823)]), AuthorCompany(id=1215295125949957022, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, xref=2, ext=[AuthorCompanyExt(id=1215295125958345629, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, companyId=1215295125949957022, language=EN, country=null, province=null, city=null, postcode=null, companyName=null, departmentName=null, remark=2School of Marine Sciences, Ningbo University, Ningbo 315823, China)]), AuthorCompany(id=1215295126012871583, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, xref=3, ext=[AuthorCompanyExt(id=1215295126021260193, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, companyId=1215295126012871583, language=CN, country=null, province=null, city=null, postcode=null, companyName=null, departmentName=null, remark=3 宁波市海洋与渔业研究院,浙江 宁波 315012)]), AuthorCompany(id=1215295126088369060, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, xref=3, ext=[AuthorCompanyExt(id=1215295126096757670, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, companyId=1215295126088369060, language=EN, country=null, province=null, city=null, postcode=null, companyName=null, departmentName=null, remark=3Ningbo Academy of Oceanology and Fishery, Ningbo 315012, China)]), AuthorCompany(id=1215295126172255148, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, xref=4, ext=[AuthorCompanyExt(id=1215295126176449453, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, companyId=1215295126172255148, language=CN, country=null, province=null, city=null, postcode=null, companyName=null, departmentName=null, remark=4 浙江万里学院 宁海海洋生物种业研究院,浙江 宁海 315604)]), AuthorCompany(id=1215295126243558320, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, xref=4, ext=[AuthorCompanyExt(id=1215295126247752625, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, companyId=1215295126243558320, language=EN, country=null, province=null, city=null, postcode=null, companyName=null, departmentName=null, remark=4Ninghai Institute of Mariculture Breeding and Seed Industry, Zhejiang Wanli University, Ninghai 315604, China)])], figs=[ArticleFig(id=1215295128642699288, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=EN, label=Fig. 1, caption=Changes in $ {{\rm {SO}}_4^{2-}} $ concentration of Sinonovacula constricta under sulfide stress

Different letters of the same type represented significant changes among different time at the same exposure concentration (p<0.05)

, figureFileSmall=us0erX/ggpxup2oVpkUjTw==, figureFileBig=cJp5W+ADtCAn5Bx1ChOkIg==, tableContent=null), ArticleFig(id=1215295128743362588, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=CN, label=图1, caption=硫化物胁迫下缢蛏血液$ {{\rm {SO}}_4^{2-}} $浓度的变化

同类型字母中不同字母表示同一胁迫浓度下不同时间点间的数据差异显著(p<0.05)

, figureFileSmall=us0erX/ggpxup2oVpkUjTw==, figureFileBig=cJp5W+ADtCAn5Bx1ChOkIg==, tableContent=null), ArticleFig(id=1215295128873386017, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=EN, label=Fig. 2, caption=Full-length cDNA sequence of the ScSULT1B1-12 gene and its deduced amino acid sequences

Red bold font indicated the initiation codon and stop codon, the shaded part indicated the conserved domain of the protein, the bold font and underlined mark indicated the PAPS binding domains; the yellow bold font and underlined mark indicated PAPS binding and dimerization domains; the blue bold font showed the catalytic active sites; the numbers on the left indicate the positions of nucleotide and amino acid

, figureFileSmall=qKTlRMzhhfKoGbzh84styQ==, figureFileBig=BZ/5/g3t5PVLW+uMJaROsg==, tableContent=null), ArticleFig(id=1215295128948883493, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=CN, label=图2, caption=ScSULT1B1-12基因全长cDNA序列及其推导的氨基酸序列

红色加粗字体为起始密码子、终止密码子;阴影部分为蛋白的保守结构域,加粗字体和下划线标注表示PAPS结合域;黄色加粗字体和下划线标注表示PAPS结合和二聚化域;蓝色加粗字体为氨基酸活性位点;左侧数字为核苷酸和氨基酸的位置

, figureFileSmall=qKTlRMzhhfKoGbzh84styQ==, figureFileBig=BZ/5/g3t5PVLW+uMJaROsg==, tableContent=null), ArticleFig(id=1215295129057935401, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=EN, label=Fig. 3, caption=Multiple alignments of the amino acid sequences of SULT1B1 in eleven animals

The green arrows indicated the catalytic active site; the red box indicated the PAPS binding domain; the blue box indicated the PAPS binding and dimerization domain; the species name and the corresponding accession numbers of the sequences used are shown in appendix Table S1

, figureFileSmall=GnpxDKH5+PFLk/Xe1yU64w==, figureFileBig=JnaxhDwdgE1KchYXJ772iA==, tableContent=null), ArticleFig(id=1215295129146015787, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=CN, label=图3, caption=11种动物SULT1B1氨基酸序列的多重比较

绿色箭头表示催化活性位点;红框表示PAPS结合域;蓝框表示PAPS结合和二聚化域;所使用序列的物种名及基因登录号见附表S1

, figureFileSmall=GnpxDKH5+PFLk/Xe1yU64w==, figureFileBig=JnaxhDwdgE1KchYXJ772iA==, tableContent=null), ArticleFig(id=1215295129238290479, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=EN, label=Fig. 4, caption=The ScSULT1B1-12 phylogenetic tree constructed by neighbor-joining method

Accession numbers of the sequences used in construction of tree are shown in appendix Table S1

, figureFileSmall=540X8EbGZkKiKZyD6P+UPQ==, figureFileBig=ef2bd5nZOrI4ZDUaXiGxAA==, tableContent=null), ArticleFig(id=1215295129309593650, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=CN, label=图4, caption=邻接法构建的ScSULT1B1-12系统进化树

所使用序列的基因登录号见附表S1

, figureFileSmall=540X8EbGZkKiKZyD6P+UPQ==, figureFileBig=ef2bd5nZOrI4ZDUaXiGxAA==, tableContent=null), ArticleFig(id=1215295129389285429, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=EN, label=Fig. 5, caption=The expression of ScSULT1B1-12 gene in different tissues of Sinonovacula constricta

Different letters represented significant changes among different tissues (p<0.05)

, figureFileSmall=9NHitFiRmQFCd9Aibz23ew==, figureFileBig=uRGGEHWTE8gTj/FExcJfGw==, tableContent=null), ArticleFig(id=1215295129489948729, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=CN, label=图5, caption= ScSULT1B1-12基因在缢蛏不同组织中的表达

不同字母表示组织间的数据差异显著(p<0.05)

, figureFileSmall=9NHitFiRmQFCd9Aibz23ew==, figureFileBig=uRGGEHWTE8gTj/FExcJfGw==, tableContent=null), ArticleFig(id=1215295129569640508, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=EN, label=Fig. 6, caption=The expression characteristics of the ScSULT1B1-12 gene in gill (M) and hepatopancreas (m) of Sinonovacula constricta under sulfide stress

Different letters of the same type represented significant changes among different time at the same exposure concentration (p<0.05)

, figureFileSmall=Ygm+f4EQxC0Hk/BPqVHf/w==, figureFileBig=5FgSnJEMGynqx0sEALogBg==, tableContent=null), ArticleFig(id=1215295129649332287, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=CN, label=图6, caption=硫化物胁迫下ScSULT1B1-12基因在缢蛏鳃(M)和肝胰腺(m)中的表达特征

同类型字母中不同字母表示同一胁迫浓度下不同时间点间的数据差异显著(p<0.05)

, figureFileSmall=Ygm+f4EQxC0Hk/BPqVHf/w==, figureFileBig=5FgSnJEMGynqx0sEALogBg==, tableContent=null), ArticleFig(id=1215295129716441154, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=EN, label=Table 1, caption=

Primers and their sequences used in the experiment

, figureFileSmall=null, figureFileBig=null, tableContent=
引物名称序列(5'-3'
SULT1B1-12-FCAAATCCGAATGGAAAGGCGG
SULT1B1-12-RCAACAGAATCTGTATGTGAAG
RS9-FTGAAGTCTGGCGTGTCAAGT
RS9-RCGTCTCAAAAGGGCATTACC
), ArticleFig(id=1215295129808715845, tenantId=1146029695717560320, journalId=1149651085930835976, articleId=1211258400625791116, language=CN, label=表1, caption=

实验所用引物及其序列

, figureFileSmall=null, figureFileBig=null, tableContent=
引物名称序列(5'-3'
SULT1B1-12-FCAAATCCGAATGGAAAGGCGG
SULT1B1-12-RCAACAGAATCTGTATGTGAAG
RS9-FTGAAGTCTGGCGTGTCAAGT
RS9-RCGTCTCAAAAGGGCATTACC
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硫化物胁迫对缢蛏血液${\rm {SO}} _4^{2-}$浓度及SULT1B1-12基因表达的影响
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孙慧妙 1, 2 , 沈伟良 3 , 陈彩芳 1, * , 林志华 1, 4 , 韩庆喜 2
海洋学报 | 论文 2023,45(1): 62-70
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海洋学报 | 论文 2023, 45(1): 62-70
硫化物胁迫对缢蛏血液${\rm {SO}} _4^{2-}$浓度及SULT1B1-12基因表达的影响
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孙慧妙1, 2 , 沈伟良3, 陈彩芳1, * , 林志华1, 4, 韩庆喜2
作者信息
  • 1 浙江万里学院 生物与环境学院 浙江省水产种质资源高效利用技术研究重点实验室,浙江 宁波 315100
  • 2 宁波大学 海洋学院,浙江 宁波 315823
  • 3 宁波市海洋与渔业研究院,浙江 宁波 315012
  • 4 浙江万里学院 宁海海洋生物种业研究院,浙江 宁海 315604
  • 孙慧妙(1996-),女,浙江省衢州市人,研究方向为滩涂贝类环境适应机制。E-mail:

通讯作者:

*陈彩芳,女,博士,副教授,硕士生导师,主要从事海洋生物环境适应性研究。E-mail:
Effects of sulfide stress on blood ${{\bf {SO}} _4^{2-}} $ concentration and SULT1B1-12 gene expression in Sinonovacula constricta
Huimiao Sun1, 2 , Weiliang Shen3, Caifang Chen1, * , Zhihua Lin1, 4, Qingxi Han2
Affiliations
  • 1Zhejiang Key Laboratory of Aquatic Germplasm Resources, College of Biological and Environmental Sciences, Zhejiang Wanli University, Ningbo 315100, China
  • 2School of Marine Sciences, Ningbo University, Ningbo 315823, China
  • 3Ningbo Academy of Oceanology and Fishery, Ningbo 315012, China
  • 4Ninghai Institute of Mariculture Breeding and Seed Industry, Zhejiang Wanli University, Ninghai 315604, China
出版时间: 2023-01-01 doi: 10.12284/hyxb2023004
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作为典型的埋栖型滩涂贝类,缢蛏(Sinonovacula constricta)常暴露在富含硫化物的环境中,并表现出较强的硫化物耐受能力。胞质磺基转移酶1B1(SULT1B1)位于硫代谢途径下游,是催化磺化反应的关键酶,在甲状腺激素(THs)等内源性物质的生物转化过程中发挥重要作用。为研究ScSULT1B1-12基因在缢蛏耐硫中的作用,本研究采用生物信息学方法分析了其序列特征,并结合血液中${\rm {SO}} _4^{2-} $浓度变化,开展其组织表达及不同浓度(50 μmol/L、150 μmol/L、300 μmol/L)硫化物胁迫72 h后的表达特征研究。结果表明,ScSULT1B1-12基因全长cDNA为1 100 bp,含有 897 bp的开放阅读框,编码298个氨基酸。序列分析表明,ScSULT1B1-12含有4个催化活性位点(56K、104N、106H和134A)、1个N端的PAPS结合域(YPKSGTXW)、1个C端的PAPS结合和二聚化域(RKGXXGDWKNXFTVXXE),表明其在结构上具有催化磺化反应的能力。组织分布表明,ScSULT1B1-12基因在鳃中高表达,其次为闭壳肌和肝胰腺。硫化物胁迫后缢蛏血液中${\rm {SO}} _4^{2-} $浓度呈下降趋势,ScSULT1B1-12基因的表达模式也在波动中呈下降趋势,表明硫酸盐可进一步被活化生成磺化反应的供体,而ScSULT1B1-12介导的磺化反应受抑制后可使缢蛏体内THs保持在一定水平,以加强其代谢机能和免疫功能,使机体适应高硫化物的不良环境。

缢蛏  /  ScSULT1B1-12  /  硫化物胁迫  /  时间表达  /  硫酸根

As a typical dwelled tidal shellfish, Sinonovacula constricta is often exposed to sulfide-rich environment and shows strong sulfide tolerance. The cytosolic sulfotransferase 1B1 (SULT1B1) is located at downstream of the sulfur metabolism pathway, while it is a key enzyme catalyzing the sulfation reaction and plays an important role in the biotransformation of endogenous substances such as thyroid hormones (THs). In order to study the role of ScSULT1B1-12 in sulfur resistance, the sequence characteristics were analyzed by bioinformatics method. Combined with the changes of blood ${\rm {SO}} _4^{2-} $ concentration, the spatial expression and temporal expression profiles during 72 h sulfide stress (50 μmol/L, 150 μmol/L, 300 μmol/L) were studied. The full-length cDNA of ScSULT1B1-12 gene was 1 100 bp, containing an open reading frame of 897 bp, and encoding 298 amino acids. Sequence analysis showed that ScSULT1B1-12 contains four catalytic active sites (56K, 104N, 106H, and 134A), one PAPS binding domain (YPKSGTXW) at N terminal, and one PAPS binding and dimerization domain (RKGXXGDWKNXFTVXXE) at C terminal, indicating that it was structurally able to catalyze the sulfation reaction. Spatial expression showed that ScSULT1B1-12 was highly expressed in gills, followed by the adductor muscle and hepatopancreas. Blood ${\rm {SO}} _4^{2-} $ concentration decreased, and the expression patterns of ScSULT1B1-12 also declined with fluctuation after sulfide stress, indicating that sulfate can be further transformed to sulfated donors, and ScSULT1B1-12-mediated sulfation may be inhibited to keep THs at a certain level in S. constricta, in order to strengthen the metabolic and immune functions, and make the organism adapt the adverse environment of high sulfide.

Sinonovacula constricta  /  ScSULT1B1-12  /  sulfide stress  /  temporal expression  /  sulfate ion
孙慧妙, 沈伟良, 陈彩芳, 林志华, 韩庆喜. 硫化物胁迫对缢蛏血液${\rm {SO}} _4^{2-}$浓度及SULT1B1-12基因表达的影响. 海洋学报, 2023 , 45 (1) : 62 -70 . DOI: 10.12284/hyxb2023004
Huimiao Sun, Weiliang Shen, Caifang Chen, Zhihua Lin, Qingxi Han. Effects of sulfide stress on blood ${{\bf {SO}} _4^{2-}} $ concentration and SULT1B1-12 gene expression in Sinonovacula constricta[J]. Haiyang Xuebao, 2023 , 45 (1) : 62 -70 . DOI: 10.12284/hyxb2023004
水生穴居动物由于生存空间有限,其摄食、排泄均在洞穴中进行,导致残饵、排泄物等有机物在洞穴中积累。尤其是退潮时,洞穴内氧气含量迅速下降,在缺氧条件下,底部沉积物中的硫酸盐、亚硫酸盐和含硫有机物会被还原为硫化物H2S[1],使得穴居动物长时间暴露于高浓度的硫化物环境中,对硫化物产生了一定的耐受性。目前对耐硫生物的研究主要集中在单环刺螠(Urechis unicinctus[2] 、美洲刺螠(Urechis caupo)[3]、罗氏沼虾(Macrobrachium rosenbergii[4]和日本沼虾(Macrobrachium nipponense[5]等水生无脊椎动物中。
硫化物(H2S、HS和S2−)是底栖环境常见的不良环境因子,具有呼吸毒性和免疫毒性[6-7],会抑制需氧生物的有氧呼吸,使新陈代谢减慢,甚至导致生物体的死亡。为了抵御硫化物的毒性,耐硫生物会对其进行氧化代谢解毒[2]。此硫化物氧化代谢途径在硫醌氧化还原酶(Sulfide Quinine Oxidoreductase,SQR)、硫双加氧酶(Sulfur Dioxygenase,SDO)、硫转移酶(Sulfur Transferases,ST)等一系列酶的作用下,将有毒硫化物转化为无毒硫酸盐[8]。硫酸盐在机体内会被进一步活化为3'-磷酸腺苷5'-磷酸硫酸(3'-phosphoadenosine-5'-phosphosulfate,PAPS);而胞质磺基转移酶(Cytosolic Sulfotransferase,SULT)以PAPS作为其磺化反应的通用供体,促进甲状腺激素、类固醇和儿茶酚胺类等有效内源性物质的失活和消除[9]。胞质磺基转移酶1B1(Cytosolic Sulfotransferase 1B1, SULT1B1)通过磺化反应调节甲状腺激素(Thyroid Hormones,THs)水平[10],以调控机体生理代谢水平。
缢蛏(Sinonovacula constricta)是我国重要的经济养殖贝类之一,常栖居于潮间带的泥砂质滩涂中。作为典型的穴居双壳贝类,其埋栖深度可达体长的5~8倍,远远深于泥蚶(Tegillarca granosa)、文蛤(Meretrix meretrix)等其他滩涂贝类[11-12]。由于潮汐作用和洞穴内有限的海水交换,缢蛏常暴露于高浓度的硫化物环境中,且其耐受硫化物的能力要强于单环刺螠、中华绒螯蟹(Eriocheir sinensis)、罗氏沼虾等水生动物[12-13]。本课题组已有研究表明,缢蛏线粒体硫化物氧化途径是其对硫化物解毒的重要策略[11-12];在对其基因组的进一步分析中发现,缢蛏SULT1B1(ScSULT1B1)基因家族存在基因扩张现象,且在对已有的硫化物胁迫后缢蛏鳃转录组数据的比较分析中亦筛选到了该家族成员SULT1B1-12基因的全长cDNA序列。因此,本研究拟以硫代谢途径中间产物—硫酸盐水平为连接点,对ScSULT1B1-12基因的序列特征、组织表达和硫化物胁迫后的表达特征进行分析,探讨其在缢蛏耐硫性状中的作用机制,旨在为缢蛏耐硫化物分子机制研究及后续开展分子标记辅助育种提供理论依据。
实验用缢蛏采集自宁波市海洋与渔业研究院科技创新基地。选取健康、活力好、壳体完整、规格均匀的成年缢蛏,体质量为(10.72±1.64)g,壳长为(5.8±0.5)cm。实验开始前暂养7 d,海水盐度为21.2±0.5,温度为(18.1±1.5)℃,连续充气,每日换水1次,并定时投喂适量的小球藻。随机选取4颗缢蛏,设为4个生物学平行,分别解剖取其鳃、闭壳肌、肝胰腺、斧足、外套膜、水管等组织,组织经液氮速冻后保存于−80℃,用于ScSULT1B1-12基因的组织表达研究。
选取384颗健康缢蛏成贝进行硫化物攻毒实验。在实验开始前2 d停止投喂和充氧。鉴于硫化物对缢蛏的96 h安全浓度为158 μmol/L [11],故本研究设置3个浓度组,分别为50 μmol/L、150 μmol/L和300 μmol/L,每组均设4个平行。实验用九水硫化钠(Na2S·9H2O)配置100 mmol/L硫化物母液,成倍稀释母液使水体浓度分别达到相应实验设定浓度。每3 h补充1次母液,以维持暴毒水体硫化物浓度的稳定。于硫化物攻毒后0 h、3 h、6 h、12 h、24 h、48 h、72 h,从各平行组随机选取4颗缢蛏,抽取血液后解剖取其鳃和肝胰腺。各样品均于液氮速冻后储存于−80℃,用于ScSULT1B1-12基因的时间表达研究。
用珠磨法破碎缢蛏血细胞,3 000 r/min离心5 min;取上清液1 mL,加入1 mL乙腈沉淀蛋白质后加入8 mL去离子水,振荡混匀后静置5 min;随后10 000 r/min离心10 min,取上清液,经过孔径为0.22 μm滤膜过滤。经离子色谱法检测滤液中${\rm {SO}} _4^{2-} $浓度。
从硫化物胁迫后缢蛏鳃转录组数据库中筛选得到ScSULT1B1-12基因全长序列。利用ORF Finder查找其开放阅读框(Open Reading Box,ORF)。使用NCBI(National Center for Biotechnology Information)的BLAST(Basic Local Alignment Search Tool)(http://www.ncbi.nlm.nih.gov/blast)分析序列的完整性并进行同源性比较分析。使用ProtParam预测其等电点(Isoelectric point,pI)和分子量(Molecular weight,Mw)(https://web.expasy.org/protparam/)。利用PROSITE(https://prosite.expasy.org/)进行功能域的分析。通过SWISS-MODEL(https://npsa-prabi.ibcp.fr/)进行其蛋白质高级结构预测。用Clustal W软件进行多序列比对分析。利用MEGA-7软件构建系统发育树,并利用iTOL(https://itol.embl.de/)进行在线美化。
Trizol法提取缢蛏组织总RNA,使用 PrimeScriptTM RT reagent Kit with gDNA Eraser(TaKaRa,日本)反转录成cDNA模板。根据ScSULT1B1-12基因全长序列设计RT-qPCR引物(表1)。利用LightCycler® 480II实时PCR系统进行荧光定量PCR反应,每组样品设4个生物学平行,4个技术重复。以RS9基因为内参基因[14],采用2−ΔΔCT[15]计算ScSULT1B1-12的相对表达量。
所有数据以平均值±标准差来表示,均使用SPSS 18.0软件进行单因素方差分析(One-way ANOVA),p<0.05表示差异显著。
随着胁迫时间的延长,除50 μmol/L浓度组外,其余较高浓度组(150 μmol/L、300 μmol/L)缢蛏血液${\rm {SO}} _4^{2-} $浓度波动较大,总体均呈下降趋势;且浓度越高,波动越剧烈(图1)。50 μmol/L硫化物胁迫下,其${\rm {SO}} _4^{2-} $浓度波动不大,在3 h时小幅上升,6 h时略微下降,随后12 h、24 h、48 h时保持上升趋势,但差异不显著(p>0.05),72 h时小幅下降。150 μmol/L硫化物胁迫下,其${\rm {SO}} _4^{2-} $浓度3 h时显著下降(p<0.05),6 h、12 h时持续小幅上升,之后24 h时有所下降,到48 h、72 h时保持在同一水平内波动。300 μmol/L硫化物胁迫下,其${\rm {SO}} _4^{2-} $浓度3 h时显著上升(p<0.05),6 h时大幅下降(p<0.05),12 h时再次显著升高(p<0.05),24 h时小幅波动,48 h、72 h持续大幅下降(p<0.05)。
ScSULT1B1-12基因的cDNA序列全长为1 100 bp,包含 897 bp的ORF,编码298个氨基酸(图2)。其预测的蛋白分子量为35.03 kDa,理论等电点为6.37,其中极性氨基酸所占比例较高,为亲水性蛋白,无信号肽。功能域预测发现其有1个功能域(Pfam:Sulfotransfer_1,46~291 aa)。该蛋白的二级结构由117个H键、137个螺旋数和44个转角组成。三级结构预测显示其为同源二聚体。
氨基酸序列同源性分析显示,ScSULT1B1-12与其他软体动物ScSULT1B1的同源性最高,其中与长牡蛎(Crassostrea gigas)和美洲牡蛎(Crassostrea virginica)的同源性分别为52.36%和48.48%。与其他动物SULT1B1进行多重序列比对表明,该基因保守性较高,含有4个催化活性位点(56K、104N、106H和134A)、N端的PAPS结合域(YPKSGTXW)、C端的PAPS结合和二聚化域(RKGXXGDWKNXFTVXXE)(图3)。
用MEGA7.0软件以邻接法构建了各物种SULT1B1的系统进化树,在线美化后如图4所示。该进化树由3个分支组成,ScSULT1B1-12首先与贝类聚为一支,随后与节肢动物聚为一支,最后再与脊椎动物聚为一支。
利用RT-qPCR技术检测了ScSULT1B1-12在缢蛏鳃、闭壳肌、肝胰腺、斧足、外套膜、水管中的表达情况(图5)。结果表明ScSULT1B1-12基因在6种组织中均有表达,且其在鳃中表达量最高,其次为闭壳肌和肝胰腺。
硫化物胁迫下,缢蛏鳃中ScSULT1B1-12基因表达水平随着时间的延长总体呈下降−升高−下降的波动模式(图6M)。50 μmol/L硫化物胁迫下,鳃 ScSULT1B1-12基因的表达量在3 h 时略微下降,6 h、12 h 时小幅波动上升后于 24 h 时显著升高(p<0.05),随后 48 h 时显著下降(p<0.05),并在 72 h 时略有上升。150 μmol/L 硫化物胁迫下,鳃 ScSULT1B1-12 基因的表达量在 3 h 时显著下降(p<0.05),6 h、12 h 时小幅波动后于 24 h 时显著升高(p<0.05),随后 48 h 时显著下降(p<0.05),并在 72 h 时保持在同一表达水平。300 μmol/L硫化物胁迫下,鳃ScSULT1B1-12基因的表达水平较前两组波动剧烈,在3 h时略微下降后于6 h时显著上升至峰值(p<0.05),12 h时显著下降(p<0.05),随后24 h小幅升高,在48 h时又剧烈下降(p<0.05),最后于72 h时保持在同一表达水平。
硫化物胁迫下,缢蛏肝胰腺中ScSULT1B1-12基因表达水平亦呈波动模式(图6m)。50 μmol/L、150 μmol/L硫化物胁迫下,肝胰腺ScSULT1B1-12基因的表达模式类似,总体呈下降趋势。50 μmol/L浓度组,其基因表达量在3 h时显著下降(p<0.05),随后在6 h、12 h、24 h、48 h时在同一范围内小幅波动,最后于72 h时显著下降(p<0.05)。150 μmol/L浓度组,肝胰腺ScSULT1B1-12基因表达量在前3 h维持同一水平,6 h时显著下降(p<0.05),之后在12 h时显著上升(p<0.05),随后24 h、48 h、72 h时保持下降趋势。300 μmol/L浓度组,肝胰腺ScSULT1B1-12基因的表达量在3 h时略微下降,6 h继续下降后于12 h、24 h、48 h时在同一范围内波动,最后于72 h小幅上升。
硫是生命的基本元素,硫代谢对细胞的生长和存活至关重要[8]。在该代谢通路中,首先硫化物相继在SQR、SDO、ST等酶的催化下氧化生成代谢中间产物硫酸盐[8]。本研究发现,硫化物胁迫后缢蛏血液${\rm {SO}} _4^{2-} $浓度与胁迫时间呈负相关关系。而硫酸盐必须经活化后才能参与SULT介导的磺化反应,并在调节内源性化学物质的生物活性,促进其消除中发挥关键作用[9, 16]。故推测硫化物胁迫后缢蛏体内硫酸盐产物被活化为PAPS,为磺化反应提供通用供体[9],在激素、儿茶酚胺神经递质等的稳态中起着重要作用[17]
SULT1B1属于SULT超家族成员之一[18]。该超家族基因包含4个保守的催化活性位点、PAPS结合域、PAPS结合和二聚化域[19]。本研究中ScSULT1B1-12基因也具有上述的催化活性位点及保守功能域。其中位于其C端的KTVE基序(KXXXTVXXE)是SULTs中同源和异源二聚体的常见蛋白质相互作用基序[20]。大多数SULTs是以同源二聚体形式存在[21]。这亦与本研究结果一致,ScSULT1B1-12蛋白的三级结构预测显示其为同源二聚体。除了SULTs的催化残基和二聚化区域外,SULTs最保守的区域是PAPS结合域[22]。每个亚型都必须结合PAPS才能发挥其功能[23]。这些活性位点与结构域为ScSULT1B1-12发挥其磺化功能提供了结构支撑。
ScSULT1B1-12基因的组织表达结果发现其主要在鳃和肝胰腺中高表达,其中鳃表达量最高。这可能是由于鳃是水生生物的呼吸器官,直接暴露于硫化物中[11],其对胁迫的敏感性较高[24];而肝胰腺作为经典的解毒代谢器官,也是硫化物氧化的主要部位[25-26]ScSULT1B1-12基因在缢蛏肝胰腺中高表达,与在啮齿动物和人类中的研究结果相一致[27],推测可能与该器官的强代谢能力有关[28-29]
SULT1B1催化以THs为底物的磺化反应[10, 30],该反应是THs代谢的重要途径[10],以调节机体内THs的稳态。而THs是机体最重要的激素之一[31],可调节所有组织的新陈代谢[10, 31-33],且能参与免疫调节[34-37]。本研究结果表明,硫化物胁迫下ScSULT1B1-12基因的转录水平呈波动模式,总体呈下降趋势。这可能是由于磺化反应是导致THs失活的重要一步[10],在胁迫初期ScSULT1B1-12基因的表达量显著升高,使THs大量失活以抑制机体的生理代谢水平,降低其能量消耗;但随着胁迫时间的延长,其表达量受抑制,可使THs活性保持在一定水平,以加强机体代谢机能来维持基本生命活动所需,同时提高机体的免疫功能,以应对高硫化物浓度的不良环境。此外,缢蛏体内${\rm {SO}} _4^{2-} $浓度的变化,从一定程度上也反应了被活化的硫酸盐通用供体,还可能参与除SULT1B1外的其他SULT超家族成员介导的磺化反应。
本研究对ScSULT1B1-12基因的序列结构进行生物信息学分析,表明其在结构上具备催化磺化反应的能力。组织分布表明,其在鳃和肝胰腺中表达量较高。硫化物胁迫后缢蛏血液${\rm {SO}} _4^{2-} $浓度呈下降趋势,同时ScSULT1B1-12基因的转录水平呈抑制趋势,表明硫酸盐可被活化生成磺化反应的供体,而ScSULT1B1-12催化的磺化反应受抑制后可使缢蛏体内THs保持活性,以加强其代谢机能来维持机体的基本生命活动,同时提高机体的免疫功能,以适应高硫化物浓度的不良环境。

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  • 浙江省公益技术应用研究项目(LGN22C190025);国家重点研发计划“蓝色粮仓”科技创新课题(2018YFD0901405,2020YFD0900802);财政部和农业农村部:国家现代农业产业技术体系项目(CARS-49);浙江省科技重点研发计划(2019C02054,2021C02069-7)。
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doi: 10.12284/hyxb2023004
  • 接收时间:2022-03-25
  • 首发时间:2025-12-26
  • 出版时间:2023-01-01
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  • 收稿日期:2022-03-25
  • 修回日期:2022-06-24
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浙江省公益技术应用研究项目(LGN22C190025);国家重点研发计划“蓝色粮仓”科技创新课题(2018YFD0901405,2020YFD0900802);财政部和农业农村部:国家现代农业产业技术体系项目(CARS-49);浙江省科技重点研发计划(2019C02054,2021C02069-7)。
作者信息
    1 浙江万里学院 生物与环境学院 浙江省水产种质资源高效利用技术研究重点实验室,浙江 宁波 315100
    2 宁波大学 海洋学院,浙江 宁波 315823
    3 宁波市海洋与渔业研究院,浙江 宁波 315012
    4 浙江万里学院 宁海海洋生物种业研究院,浙江 宁海 315604

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*陈彩芳,女,博士,副教授,硕士生导师,主要从事海洋生物环境适应性研究。E-mail:
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2种不同金属材料的力学参数

Family
属数
Number of
genus
种数
Number of
species
占总种数比例
Percentage of
total species (%)

Genus
种数
Number of
species
占总种数比例
Percentage of total
species (%)
鹅膏菌科Amanitaceae 2 11 5.26 鹅膏菌属 Amanita 10 4.78
小菇科 Mycenaceae 2 12 5.74 丝盖伞属 Inocybe 5 2.39
多孔菌科 Polyporaceae 8 14 6.70 蜡蘑属 Laccaria 5 2.39
红菇科 Russulaceae 3 23 11.00 小皮伞属 Marasmius 6 2.87
小菇属 Mycena 11 5.26
光柄菇属 Pluteus 5 2.39
红菇属 Russula 17 8.13
栓菌属 Trametes 5 2.39
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