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Tandem Repeats High Copy Number and Remarkable Diel Expression Rhythm of Form II RuBisCO in Prorocentrum donghaiense (Dinophyceae)

机译:东海原螯虾(Rinoiscent donghaiense(Dinophyceae))II型RuBisCO的串联重复序列高拷贝数和显着的Diel表达节奏

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摘要

Gene structure and expression regulation of form II RuBisCO (rbcII) in dinoflagellates are still poorly understood. Here we isolated this gene (Pdrbc) and investigated its diel expression pattern in a harmful algal bloom forming dinoflagellate Prorocentrum donghaiense. We obtained cDNA sequences with triple tandem repeats of the coding unit (CU); the 5′ region has the sequence of a typical dinoflagellate plastid gene, encoding an N-terminus with two transmembrane regions separated by a plastid transit peptide. The CUs (1,455 bp except 1464 bp in last CU) are connected through a 63 bp spacer. Phylogenetic analysis showed that rbcII CUs within species formed monophyletic clusters, indicative of intraspecific gene duplication or purifying evolution. Using quantitative PCR (qPCR) we estimated 117±40 CUs of Pdrbc in the P. donghaiense genome. Although it is commonly believed that most dinoflagellate genes lack transcriptional regulation, our RT-qPCR analysis on synchronized cultures revealed remarkable diel rhythm of Pdrbc expression, showing significant correlations of transcript abundance with the timing of the dark-to-light transition and cell cycle G2M-phase. When the cultures were shifted to continuous light, Pdrbc expression remained significantly correlated with the G2M-phase. Under continuous darkness the cell cycle was arrested at the G1 phase, and the rhythm of Pdrbc transcription disappeared. Our results suggest that dinoflagellate rbcII 1) undergoes duplication or sequence purification within species, 2) is organized in tandem arrays in most species probably to facilitate efficient translation and import of the encoded enzyme, and 3) is regulated transcriptionally in a cell cycle-dependent fashion at least in some dinoflagellates.
机译:在鞭毛鞭毛虫中,II型RuBisCO(rbcII)的基因结构和表达调控尚不清楚。在这里,我们分离了该基因(Pdrbc),并在有害藻华中形成了鞭毛藻(Diroflagellate dongroense),研究了其diel表达模式。我们获得了具有编码单元(CU)三重串联重复序列的cDNA序列。 5'区域具有典型的鞭毛藻体质体基因的序列,其编码具有由质体转运肽隔开的两个跨膜区的N端。 CU(最后一个CU中的1464 bp除外,为1,455 bp)通过63 bp的垫片连接。系统发育分析表明,物种内的rbcII CU形成了单系簇,表明种内基因重复或纯化进化。使用定量PCR(qPCR),我们估计了东海疟原虫基因组中Pdrbc的117±40 CU。尽管通常认为大多数鞭毛鞭毛藻基因缺乏转录调控,但我们对同步培养的RT-qPCR分析显示Pdrbc表达具有明显的迪尔节奏,表明转录本丰度与暗光过渡时间和细胞周期G2M密切相关-相。当培养物转移到连续光照下时,Pdrbc表达仍与G2M期显着相关。在连续黑暗中,细胞周期停滞在G1期,Pdrbc转录的节奏消失了。我们的结果表明,鞭毛鞭毛虫rbcII 1)在物种内进行重复或序列纯化,2)在大多数物种中以串联阵列形式组织,可能有助于有效翻译和导入编码的酶,3)在细胞周期依赖性细胞中受转录调控至少在一些鞭毛虫中流行。

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