α-copaene | 947-59-1
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物化性质
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计算性质
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ADMET
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安全信息
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SDS
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制备方法与用途
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上下游信息
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文献信息
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表征谱图
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同类化合物
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相关功能分类
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相关结构分类
物化性质
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熔点:74 °C
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比旋光度:D22 -6.3° (c = 1.20 in chloroform)
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沸点:124 °C15 mm Hg(lit.)
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密度:0.910 g/mL at 20 °C(lit.)
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溶解度:氯仿(微溶)、甲醇(微溶)
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LogP:5.710
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稳定性/保质期:如果按照规格使用和储存,则不会分解,未有已知危险发生。
计算性质
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辛醇/水分配系数(LogP):4.5
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重原子数:15
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可旋转键数:1
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环数:4.0
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sp3杂化的碳原子比例:0.87
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拓扑面积:0
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氢给体数:0
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氢受体数:0
制备方法与用途
α-蒎烯是合成冰片、樟脑、松油醇、二氢月桂烯醇及其他香料产品的原料之一,也是松节油的主要成分。松节油是以富含松脂的松树为原料,通过不同的加工方式得到的一种具有芳香气味的萜烯混合液。
应用由于α蒎烯独特的环状结构和双键结构,它可以通过环氧化、加成、异构化等反应合成萜烯醇、芳香醇等多种重要的有机化学品,展现出极其广泛的应用前景。
上下游信息
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下游产品
中文名称 英文名称 CAS号 化学式 分子量 (1S,4aS,8aR)-1-异丙基-4,7-二甲基-1,2,4A,5,6,8A-六氢萘 (-)-α-muurolene 10208-80-7 C15H24 204.356 (1S,8aR)-1-异丙基-4,7-二甲基-1,2,3,5,6,8a-六氢萘 delta-cadinene 483-76-1 C15H24 204.356
反应信息
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作为反应物:参考文献:名称:Polovinka, M. P.; Mamatyuk, V. I.; Korchagina, D. V., Journal of Organic Chemistry USSR (English Translation), 1991, vol. 27, # 5.2, p. 863 - 882摘要:DOI:
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作为产物:参考文献:名称:Biosynthesis and Emission of Terpenoid Volatiles from Arabidopsis Flowers摘要:人们认为拟南芥主要通过自花授粉繁殖,但一些遗传和形态学证据表明,在野生种群中,至少存在低频的昆虫介导异花授粉现象。本文中,我们展示了拟南芥花朵会释放单萜和倍半萜,这些物质可能是授粉昆虫的嗅觉线索。在拟南芥基因组中的32个萜烯合成酶基因中,有20个在花朵中表达,其中6个仅在花朵中表达或几乎仅在花朵中表达。我们对两个仅在花朵中表达的萜烯合成酶基因和一个几乎仅在花朵中表达的萜烯合成酶基因进行了表征,发现它们编码的蛋白能够催化主要花挥发物的形成。通过构建一个带有其中一种基因启动子的β-葡萄糖醛酸酶融合表达载体,我们发现基因表达仅限于萼片、柱头、花药丝和花托,当柱头接受异花授粉时,基因表达达到峰值。拟南芥花朵合成并释放挥发物的现象引发了人们对拟南芥野生繁殖行为的兴趣,并使得人们能够利用这种模式植物系统对花挥发物的生物合成及其调控进行详细研究。DOI:10.1105/tpc.007989
文献信息
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Identification, functional characterization and developmental regulation of sesquiterpene synthases from sunflower capitate glandular trichomes作者:Jens C Göpfert、Gillian MacNevin、Dae-Kyun Ro、Otmar SpringDOI:10.1186/1471-2229-9-86日期:——steps of sesquiterpene lactone biosynthesis. Reverse transcription-PCR experiments led to the identification of three sesquiterpene synthases. By combination of in vitro and in vivo characterization of sesquiterpene synthase gene products in Escherichia coli and Saccharomyces cerevisiae, respectively, two enzymes were identified as germacrene A synthases, the key enzymes of sesquiterpene lactone biosynthesis背景倍半萜内酯是菊科(或菊科)的特征代谢物,其通常表现出有效的生物活性,并被隔离在特殊器官中,例如乳管、树脂管和毛状体。对于向日葵倍半萜合酶的表征,我们采用了一种简单的方法从花药附属物中分离出纯毛状体,这有助于这些基因的鉴定和在毛状体发育过程中它们的酶功能和表达模式的研究。结果分离向日葵腺毛(Helianthus annuus L.),并提取其RNA以研究倍半萜内酯生物合成的初始步骤。逆转录-PCR 实验导致了三种倍半萜合酶的鉴定。通过分别对大肠杆菌和酿酒酵母中倍半萜烯合酶基因产物的体外和体内表征,鉴定出两种酶为倍半萜内酯生物合成的关键酶——胚芽烯 A 合酶。由于体外活性非常低,第三种酶在酵母中作为硫氧还蛋白融合蛋白在体内表达用于功能表征。在体内试验中,它被鉴定为一种多产物酶,其中挥发性倍半萜烃 delta-cadinene 是两种主要产物之一,α-muuorlene、β-石竹烯、α-葎草烯和
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Two sesquiterpene synthases are responsible for the complex mixture of sesquiterpenes emitted from Arabidopsis flowers作者:Dorothea Tholl、Feng Chen、Jana Petri、Jonathan Gershenzon、Eran PicherskyDOI:10.1111/j.1365-313x.2005.02417.x日期:2005.4
Summary Despite the fact that Arabidopsis is largely self‐pollinating, its flowers emit a complex mixture of terpene volatiles consisting predominantly of a large group of over 20 sesquiterpenes. Here we report that only two terpene synthases, encoded by the florally expressed genes
At5g23960 andAt5g44630 , are responsible for the formation of virtually all sesquiterpenes found in the Arabidopsis floral volatile blend. Two independent mutant lines with T‐DNA insertions in the previously identifiedAt5g23960 gene lacked the emission of three sesquiterpenes, including the main sesquiterpene volatile (E )‐β ‐caryophyllene, confirming the previousin vitro functional assignment for this gene. Flowers of a mutant line carrying a T‐DNA insertion in geneAt5g44630 emitted these three sesquiterpenes, but did not emit any of the remaining sesquiterpene volatiles. AnAt5g44630 cDNA was expressed inEscherichia coli and the produced protein catalyzed the conversion of farnesyl diphosphate into over 15 sesquiterpenes in similar proportions to those found in the floral volatile blend.At5g23960 andAt5g44630 promoter‐β ‐glucuronidase (GUS) fusion experiments demonstrated that both genes are expressed in several parts of the Arabidopsis flower, with strongAt5g23960 promoter‐GUS activity in the stigma and strong expression ofAt5g44630 in intrafloral nectaries. Given the previously reported antimicrobial activity of terpenes, their production in stigmas and nectaries may serve to inhibit microbial infection at these vulnerable sites. A survey of 37Arabidopsis thaliana ecotypes revealed quantitative, but almost no qualitative, variations of floral monoterpene and sesquiterpene emissions suggesting that floral terpene volatiles must play some significant role in the life of the Arabidopsis plant.摘要尽管拟南芥在很大程度上是自花授粉的,但它的花却能散发出复杂的萜烯挥发物混合物,主要由 20 多种倍半萜组成。在这里,我们报告了只有两个萜烯合成酶(由花卉表达基因 At5g23960 和 At5g44630 编码)负责拟南芥花卉挥发性混合物中几乎所有倍半萜的形成。在先前确定的 At5g23960 基因中插入 T-DNA 的两个独立突变株缺乏三种倍半萜的释放,其中包括主要的倍半萜挥发物 (E)-β-石竹烯,这证实了先前对该基因的体外功能分配。基因 At5g44630 中携带 T-DNA 插入物的突变品系的花会释放出这三种倍半萜,但不会释放出任何其余的倍半萜挥发物。At5g44630 cDNA 在大肠杆菌中表达,产生的蛋白质催化二磷酸法尼酯转化为超过 15 种倍半萜,其比例与花香挥发混合物中的比例相似。At5g23960 和 At5g44630 启动子-β-葡萄糖醛酸酶(GUS)融合实验表明,这两个基因在拟南芥花的多个部位都有表达,其中 At5g23960 启动子-GUS 在柱头有很强的活性,而 At5g44630 则在花内蜜腺有很强的表达。鉴于之前报道的萜类化合物的抗菌活性,在柱头和蜜腺中产生萜类化合物可能有助于抑制这些脆弱部位的微生物感染。对 37 个拟南芥生态型的调查显示,花单萜烯和倍半萜烯的排放量存在数量上的差异,但几乎没有质量上的差异,这表明花萜烯挥发物在拟南芥植物的生命中一定扮演着重要角色。 -
Biosynthesis and Emission of Terpenoid Volatiles from Arabidopsis Flowers作者:Feng Chen、Dorothea Tholl、John C. D'Auria、Afgan Farooq、Eran Pichersky、Jonathan GershenzonDOI:10.1105/tpc.007989日期:2003.2Arabidopsis is believed to be mostly self-pollinated, although several lines of genetic and morphological evidence indicate that insect-mediated outcrossing occurs with at least a low frequency in wild populations. Here, we show that Arabidopsis flowers emit both monoterpenes and sesquiterpenes, potential olfactory cues for pollinating insects. Of the 32 terpene synthase genes in the Arabidopsis genome, 20 were found to be expressed in flowers, 6 of these exclusively or almost exclusively so. Two terpene synthase genes expressed exclusively in the flowers and one terpene synthase gene expressed almost exclusively in the flowers were characterized and found to encode proteins that catalyze the formation of major floral volatiles. A β-glucuronidase fusion construct with a promoter of one of these genes demonstrated that gene expression was restricted to the sepals, stigmas, anther filaments, and receptacles, reaching a peak when the stigma was receptive to cross pollen. The observation that Arabidopsis flowers synthesize and emit volatiles raises intriguing questions about the reproductive behavior of Arabidopsis in the wild and allows detailed investigations of floral volatile biosynthesis and its regulation to be performed with this model plant system.人们认为拟南芥主要通过自花授粉繁殖,但一些遗传和形态学证据表明,在野生种群中,至少存在低频的昆虫介导异花授粉现象。本文中,我们展示了拟南芥花朵会释放单萜和倍半萜,这些物质可能是授粉昆虫的嗅觉线索。在拟南芥基因组中的32个萜烯合成酶基因中,有20个在花朵中表达,其中6个仅在花朵中表达或几乎仅在花朵中表达。我们对两个仅在花朵中表达的萜烯合成酶基因和一个几乎仅在花朵中表达的萜烯合成酶基因进行了表征,发现它们编码的蛋白能够催化主要花挥发物的形成。通过构建一个带有其中一种基因启动子的β-葡萄糖醛酸酶融合表达载体,我们发现基因表达仅限于萼片、柱头、花药丝和花托,当柱头接受异花授粉时,基因表达达到峰值。拟南芥花朵合成并释放挥发物的现象引发了人们对拟南芥野生繁殖行为的兴趣,并使得人们能够利用这种模式植物系统对花挥发物的生物合成及其调控进行详细研究。
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Molecular cloning and characterization of (+)-epi-α-bisabolol synthase, catalyzing the first step in the biosynthesis of the natural sweetener, hernandulcin, in Lippia dulcis作者:Mohamed Attia、Soo-Un Kim、Dae-Kyun RoDOI:10.1016/j.abb.2012.07.010日期:2012.11potential. However, the biosynthesis of hernandulcin in L. dulcis remains unknown. The first biochemical step of hernandulcin is the synthesis of (+)-epi-α-bisabolol from farnesyl diphosphate, which is presumed to be catalyzed by a unique sesquiterpene synthase in L. dulcis. In order to decipher hernandulcin biosynthesis, deep transcript sequencings (454 and Illumina) were performed, which facilitated theHernandulcin是一种C15倍半萜烯酮,是从Lippia dulcis的叶子中分离出来的天然甜味剂。由于其安全性和低热量潜力,它是一种有前途的糖替代品。但是,尚不清楚L. dulcis中hernandulcin的生物合成。Hernandulcin的第一步生化步骤是由法呢基二磷酸酯合成(+)-epi-α-bisabolol,据推测是由唯一的倍半萜中的倍半萜烯合酶催化的。为了破译hernandulcin的生物合成,进行了深转录本测序(454和Illumina),这有助于从L. dulcis克隆五个新的倍半萜烯合酶cDNA。在酵母中对这些cDNA的体内活性评估确定它们为α-copaene/δ-cadinene,双环大金花烯,β-石竹烯,反式-α-佛手柑和α-bisabolol的倍半萜烯合酶。在摇瓶培养中,工程酵母可以合成大量(〜0.3 mg / mL)的α-bisabolol。这种有效的
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Polovinka, M. P.; Mamatyuk, V. I.; Korchagina, D. V., Journal of Organic Chemistry USSR (English Translation), 1991, vol. 27, # 5.2, p. 863 - 882作者:Polovinka, M. P.、Mamatyuk, V. I.、Korchagina, D. V.、Sal'nikov, G. E.、Gatilov, Yu. V.、et al.DOI:——日期:——
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