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¡¶¼¯ÃÀ´óѧѧ±¨£¨×ÔÈ»¿Æѧ°æ£©¡·[ISSN:1007-7405/CN:35-1186/N]

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ÆÚÊý:

2022ÄêµÚ5ÆÚ

Ò³Âë:

392-400

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2022-09-28

ÎÄÕÂÐÅÏ¢/Info

Title:

Construction of Expression Vector and Expression Analysis of Rnd1 Gene in Larimichthys crocea

×÷Õß:

ÖìÅô·É1; 2; ÀîÔóÓî1; 2; ´ÞÏþÓ¨1; 2; ÍõÖ¾ÓÂ1; 2; ÀîÍ겨1; 2

(1.¼¯ÃÀ´óѧˮ²úѧԺ£¬¸£½¨ ÏÃÃÅ 361021£»2.ũҵũ´å²¿¶«º£º£Ë®½¡¿µÑøÖ³ÖصãʵÑéÊÒ£¬¸£½¨ ÏÃÃÅ 361021£©

Author(s):

ZHU Pengfei1; 2; LIZeyu1; 2; CUI Xiaoying1; 2; WANG Zhiyong1; 2; LI Wanbo1; 2

£¨1.Fisheries College,Jimei University,Xiamen 361021,China;2.Key Laboratory of Healthy Mariculture for the East China Sea,Ministry of Agriculture and Rural Affairs,Xiamen 361021,China£©

¹Ø¼ü´Ê:

´ó»ÆÓã; Rnd1»ùÒò; ±í´ï·ÖÎö; Ô­ºË±í´ï

Keywords:

large yellow croaker (Larimichthys crocea); Rnd1 gene; expression analysis; prokaryotic expression

·ÖÀàºÅ:

-

DOI:

-

ÎÄÏ×±êÖ¾Âë:

A

ÕªÒª:

Ϊ̽¾¿Rnd1»ùÒòÔÚ´ó»ÆÓãÃâÒßÓ¦´ð¹ý³ÌÖеÄ×÷Ó㬲ÉÓÃʵʱӫ¹â¶¨Á¿PCR¼¼Êõ£¨qRT-PCR£©¶Ô¸Ã»ùÒòµÄ±í´ïģʽ½øÐзÖÎö£¬Í¬Ê±¹¹½¨Ô­ºË±í´ïÔØÌåpET-28a-Rnd1£¬²¢×ª»¯½ø´ó³¦¸Ë¾úºóÓÕµ¼¸Ãµ°°×µÄÈںϱí´ï¡£Ñо¿½á¹û±íÃ÷£º´ó»ÆÓãRnd1»ùÒòORFΪ699 bp£¬±àÂë232¸ö°±»ùË᣻¾­ÐòÁжàÖرȶԺͽø»¯Ê÷¹¹½¨·¢ÏÖ£¬Rnd1µÄ°±»ùËáÐòÁи߶ȱ£ÊØ£»ÔÚ½¡¿µ´ó»ÆÓãµÄ8¸öÃâÒß×éÖ¯ÖУ¬Rnd1ÔÚ¸ÎÔàÖÐÏà¶Ô±í´ïÁ¿×î¸ß£¬Æä´ÎΪÄÔ£¬¶øÔÚ³¦Öбí´ïÁ¿×îµÍ£»±äÐμٵ¥°û¾ú¹¥¶¾ºó£¬Rnd1ÔÚ¸ÎÔàÖÐ48 hʱ´ïµ½×î¸ßÖµ£¬Îª¶ÔÕÕ×éµÄ25±¶£»ÔÚÆ¢ÔàÖÐÔò³ÖÐøÉϵ÷±í´ï£¬ÓÈÆäÔÚ48 hºóÉý¸ß¸üΪÃ÷ÏÔ¡£

Abstract:

RNA sequencing was performed on the spleen samples of Larimichthys crocea challenged by Pseudomonas plecoglossicid in our previous study.We found that the Rnd1 gene was significantly up-regulated in the samples with relatively high bacterial load compared to those with relatively low bacterial load through differential gene expression analysis.The results suggested that this gene might play an important role in the infection of P.plecoglossicid to the L.crocea.In order to explore the function of Rnd1 in the immune response of L.crocea,the expression pattern of Rnd1ª«gene was analyzed by quantitative real-time PCR (qRT-PCR)£¬and the prokaryotic expression vector of pET-28a-Rnd1ª«was constructed to express the fusion protein in E.coli.The results showed that the full-length ORF of Rnd1ª« was 699 bp,encoding 232 amino acids.Multiple sequence alignment and evolutionary tree results showed that the amino acid sequence of Rnd1 was highly conserved.The expression level of Rnd1 gene was the highest in liver£¬followed by brain£¬and the lowest expression was observed in intestine among the eight examined tissues.The relative expression of Rnd1 gene peaked at 48h in liver after stimulated by P.plecoglossicid,which was 25 times as the control group.The gene expression of Rnd1 in spleen was continuously upregulated£¬especially after 48h of the infection.

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¸üÐÂÈÕÆÚ/Last Update: 2022-11-18