米曲霉中的紫草色素诱导物对滇紫草细胞代谢的影响

在滇紫草细胞培养第８天时加入来源于米曲霉的紫草色素诱导物,１２ｈ后滇紫草细胞中紫草色素含量增加,其衍生物之一的乙酰紫草素的相对含量增加,胞内可溶蛋白合成量上升,细胞对碳源消耗增多,而细胞生长受到抑制。处理１２ｈ后,培养液电导率下降,ｐＨ上升,Ｋ＾＋外泄和Ｎａ＾＋大量内流,表明离子跨膜运输发生改变。     

真菌诱导物在滇紫草细胞培养中对紫草色素形成的影响

在滇紫草细胞悬浮培养中,真菌诱导物可抑制细胞生长,促进紫草色素的合成。将培养６ｄ的曲霉菌丝体的粗提物以６００μｇ碳水化合物／５０ｍｌ培养液的浓度加入到处于指数生长初期的滇紫草细胞悬浮培养物中,诱导物促进紫草色素合成的作用最大,紫草色素含量为对照的两倍。经高压锅处理２０ｍｉｎ到２ｈ不影响诱导物的活性。真菌诱导物还影响了紫草色素各衍生物的相对含量。     

真菌诱导物在滇紫草细胞培养中对紫草色素形成的影响

在滇紫草细胞悬浮培养中,真菌诱导物可抑制细胞生长,促进草色素的合成,将培养６ｄ的曲霉菌丝体的粗提物以６００μｇ碳水化合物／５０ｍｌ培养液的浓度加入到处于指数生长初期的滇紫草细胞悬浮培养物中,诱导物促进紫草色素合成的作用最大,紫草色素含量为对照的两倍,经高压锅处理２０ｍｉｎ到２ｈ不影响诱导物的活性,真菌诱导物还影响了紫草色素各衍生物的相对含量。     

激光和磁场对滇紫草愈伤组织色素含量的影响

用Ｈｅ－Ｎｅ激光和一定强度的磁场处理滇紫草愈伤组织,发现２～３ｈ激光辐照可提高色素含量;而１．０Ｔ磁场能促进细胞生长和色素形成,硅胶薄层层析比较两种物理因子对紫草色素成分无显著影响。     

米曲霉激发子促进紫草色素合成中细胞内Ca^2＋和cAMP的变化（简报）

米曲霉激发子促进滇紫草细胞合成紫草色素,这种作用与细胞内Ca(2 )相对浓度下降相关。离子载体A23187有抑制激发子的作用,Ca(2 )通道阻断剂Verapamil可部分模拟采曲霉激发子的作用,促进紫草色素合成。激发子处理后,胞内cAMP浓度快速上升。     

激光和磁场对滇紫草愈伤组织色素含量的影响

用He-Ne激光和一定强度的磁场处理滇紫草愈伤组织,发现2~3h激光辐照可提高色素含量;而1.0T磁场能促进细胞生长和色素形成。硅胶薄层层析比较两种物理因子对紫草色素成分无显著影响。     

真菌诱导物对滇紫草细胞色素形成的影响（简报）

在滇紫草细胞培养中加入真菌诱导物后紫草色素的合成增强,培养液的电导率和pH值在24h内分别下降和上升,且三者均以指数生长初期加入时作用最为明显。     

γ—射线对滇紫草细胞产生色素的影响

应用５００～２５００伦琴（Ｒ）的６０钴γ射线照射滇紫草（ＯｎｏｓｍａｐａｎｉｃｕｌａｔｕｍＢｕｒ．ｅｔＦｒａｎｃｈ．）细胞系,确定了应用γ射线处理促进紫草素合成的最适辐照剂量为１５００Ｒ,处理后的细胞系在生产培养基上培养２１ｄ后紫草素含量（以干重计）达到９４．７９ｍｇ／ｇ,较对照提高了１４４６％,通过小团块选种法从中筛选到了色素含量（以干重计）高达１０３．４２ｍｇ／ｇ的高产细胞系Ｍｕｔ１,其营养生长与对照相比没有差别。     

滇紫草培养细胞中色素合成的代谢调节

培养基中分别加入浓度为10^-5mol／L的铜离子,滇紫草愈伤组织中色素含量提高了5．5倍,悬浮细胞中色素含量提高8．1倍。细胞培养第21天,加入浓度为10^-5mol／L的L-Phe,色素的合成量最大。浓度为10^-6mol／L的抗坏血酸,能明显地促进培养细胞中色素的合成。     

外循环气升式反应器培养新疆紫草细胞

采用两步培养法进行新疆紫草细胞悬浮培养及5L外循环气升式反应器扩大培养,探讨了培养过程中细胞生长、紫草色素合成与培养液的电导率、可溶性糖含量变化之间的关系。第一步培养时细胞生长迅速,但也有一部分色素合成,电导率及可溶性糖含量迅速下降;第二步培养初期电导率也开始下降,但当色素合成达到高峰并有一部分外泌到培养基后,电导率又开始回升。可溶性糖捎耗很快,到后期巳测不出其存在。因此通过监测培养液中电导率及可溶性糖的变化情况,可以为新疆紫草细胞大规模培养与色素合成提供有用的参数指标。     

米根霉诱导因子对紫草细胞培养中紫草宁色素分泌的影响

在紫草细胞培养中,加入采根霉粗提物可显著提高紫草宁色素产量,并可加快胞内色素分泌到培养液中的速率和数量。在细胞培养的第6天加入米根霉诱导因子时,其促进紫草宁色素分泌的作用最大,培养液中紫草宁色素含量是对照的2．24倍。此外,同时加入正十六烷和米根霉诱导因子对紫草宁色素的分泌具有协同作用。     

The effects of CA2+ during the elicitation of shikonin derivatives inOnosma paniculatum cells

Summary A fungal elicitor extracted fromAspergillus oryzae (Ahlb.) Cobn mycelia promoted the production of shikonin derivatives inOnosma paniculatum Bur et Franch cell suspension cultures. Elicitor treatment also increased Ca²⁺ concentration in RM₉ medium, which could be measured earlier than the elicited increase of shikonin formation. Several reagents known to induce Ca²⁺-influx and increase the intracellular-free Ca²⁺ level, such as the addition of Ca (NO₃)₂·4H₂O, the Ca²⁺ ionophore A₂₃₁₈₇, and abscisic acid (ABA), appreciably suppressed the elicitor-promoted shikonin formation inOnosma cells. In contrast, the decrease of intracellular-free Ca²⁺ level by the specific Ca²⁺-chelator ethylene glycol bis (β-aminoethylether)-N,N,N′,N′-tetraacetic acid (EGTA) or the Ca²⁺—channel blocker, verapamil, enhanced the biosynthesis of shikonin even in the absence of elicitor. Treatment of cells with trifluoperazine (TFP) also stimulated shikonin formation inOnosma cell cultures. A rapid and transient drop of free Ca²⁺ level in one protoplast was directly determined after the addition of elicitor toOnosma cell cultures. The inhibitory effect on shikonin formation by ABA was largely on account of its ability to restore the intracellular Ca²⁺ level lowered by the elicitor. These results suggest that Ca²⁺ play a significant role in an early stage of the elicitation process ofOnosma cells. The rapid drop of cytoplasmic Ca²⁺ carries the elicitor signal and in turn regulates the biosynthesis of shikonin derivatives.     

稻瘟菌糖蛋白激发子诱导的水稻叶片膜脂过氧化及过敏性反应

将稻瘟菌细胞壁来源的专化性糖蛋白激发子接种于一套水稻抗稻瘟病近等基因系后,非亲和性互作水稻超氧阴离子(O-.2)积累在互作早期明显高于亲和性互作水稻;超氧化物歧化酶(SOD)和过氧化氢酶(CAT)活性均趋于下降,不同亲和性互作水稻间的差异不明显;脂氧合酶(LOX)活性在水稻/激发子非亲和互作早期增加明显、速度快;这些指标的变化进而导致非亲和性互作水稻的膜脂过氧化,其相对电导率及丙二醛(MDA)含量的高峰期和强度也明显早于和高于亲和性互作水稻.非亲和性互作水稻过氧化物酶(POD)活性在互作早期明显高于亲和性互作水稻,可能与其参与其它抗性有关.研究同时表明,激发子可专化性诱导完全和高度非亲和性互作水稻的过敏性坏死反应;而中度非亲和性互作和亲和性互作水稻则未发生过敏性(HR)坏死反应.这些结果表明,膜脂过氧化和HR反应的发生是激发子诱导水稻抗性的主要生理机制之一.     

真菌诱导子与吸附树脂对新疆紫草毛状根中萘醌积累的影响

通过考察真菌诱导子与吸附树脂对新疆紫草毛状根中萘醌积累的影响,获得真菌诱导子与吸附树脂对萘醌类物质积累的最佳处理,为规模化生产提供依据.以新疆紫草毛状根为试验材料,将黑曲霉、米曲霉诱导子及其混合诱导子、大孔吸附树脂添加到M-9培养基中,采用分光光度法测定毛状根总萘醌含量.试验结果表明:在毛状根培养10d时以2.5∶50的比例添加混合诱导子,总萘醌含量是对照的2.28倍;在此结果基础上,在培养第0天添加大孔吸附树脂NKA-9,总萘醌含量最高是对照的3.71倍;黑曲霉诱导子与米曲霉诱导子有协同效应;在生物反应器中添加混合诱导子及大孔吸附树脂NKA-9,其总萘醌含量是对照的4.17倍.米曲霉诱导子、混合诱导子对毛状根增殖有促进作用;同时添加大孔吸附树脂NKA-9及混合诱导子能提高毛状根总萘醌含量.生物反应器培养毛状根为今后利用新疆紫草毛状根规模化生产总萘醌提供了理论参考.     

Fractionation and Biological Activity of Aspergillus oryzae Elicitor Promoting Biosynthesis of Shikonin Derivatives

The Aspergillus oryzae elicitor was extracted from mycelia. The concentrated crude preparation of which was treated through DEAE-Cellulose, Sepharose-4B. Bio-Gel p- 4 and 732 columns. Elicitor activity was associated with fraction F Ⅰ b2-H, which had no affinity for DEAE-Cellulose and 732 resin. Its molecular weight was 1200～2200 D and its carbohydrate content was 6.7% of that of the crude. The elicitor activity was 120 times higher than that of crude preparation. There were also fractions F Ⅱ of nucleic acids and F Ⅰ b2-Na of nucleotides, amino acids in crude elicitor preparation. They did not affect shikonin derivative formation at low concentration, but inhibited shikonin derivative formation at high concentration. Fraction FIa of polysaccharid nature in the crude preparation which strongly inhibited shikonin derivative formation was another kind of elicitor of a new metabolite yellow pigment.     

Enhanced rosmarinic acid production by Lavandula vera MM cell suspension culture through elicitation with vanadyl sulfate

The influence of elicitation on rosmarinic acid biosynthesis by Lavandula vera MM cell suspension culture was investigated using vanadyl sulfate as an abiotic elicitor. It was established that 12 h after treatment with 25 mg/l vanadyl sulfate the rosmarinic acid production was increased up to 3.92 g/l (2.8 times higher compared to the control cultivation). No significant amounts of rosmarinic acid were detected in the culture medium in comparison with its intracellular content. However, it was observed that the extracellular content of rosmarinic acid is 3.3 times higher compared to the control variant (4 h after treatment at elicitor concentration 25 mg/l).     

Early Responses in Methyl Jasmonate-Preconditioned Cells toward Pathogen-Derived Elicitors

Early, signal transduction-related responses in cultured tobacco cells due to methyl jasmonate (MeJa), a cell-wall-derived elicitor from Phytophthora nicotianae and chitosan, were investigated. MeJa was an effective inducer of lipid peroxidation and lipoxygenase (LOX) activity with maximum levels reached within 2 h and 4–8 h, respectively. Chitosan and the elicitor induced a transient increase (1–4 h) in lipid peroxidation. Conditioning with MeJA, followed by secondary elicitation, led to a significant increase in malondialdehyde concentration after 1 h. Chitosan and the elicitor induced transient activation of LOX with maximal values between 8 and 12 h, with preconditioning resulting in a rapid increase in LOX activity at 4 h post elicitation. MeJA did not effect phosphoprotein accumulation but conditioning led to the potentiation and differential induction of phosphoproteins due to chitosan and elicitor. The results indicate that cells are sensitized by the exposure to MeJa to respond more intensely and rapidly toward secondary elicitation by fungal pathogen derived elicitors.     

The Effective Production of Shikonin by Cultures with an Increased Cell Population

We have studied the efficient production of shikonin derivatives by suspension cultures of Lithospermum erythrorhizon with an increased cell population. The yield of shikonin derivatives was highest (800 mg/liter) when 2.8 g dry wt/liter of the cells was inoculated into the M-2 medium which we had developed for the production, but the excess inoculum lowered the yield.

We investigated suitable conditions for production with the increased cell population. The optimum amount of inoculum rose to 4.9 g dry wt/liter when the concentrations of all the components contained in the M-8 medium, which we developed for increasing the productivity by modification of the M-2 medium, were increased in proportion to the amount of inoculum, and consequently we could increase the yield of the shikonin derivatives from 1400 mg/liter to 1900 mg/liter. Moreover, the increased rate of oxygen supply in addition to the enrichment of the medium made it possible to produce 2300 mg/liter of the shikonin derivatives from a culture for which 5.6 g dry wt/liter of the cells was inoculated.     

Accumulation of 2,5-dimethoxy-1,4-benzoquinone in suspension cultures of Panax ginseng by a fungal elicitor preparation and a yeast elicitor preparation

Suspension cultures of Panax ginseng C.A. Meyer (Araliaceae) were treated with either an elicitor preparation from the culture broth of the phytopathogenic hyphomycete Botrytis cinerea or a yeast elicitor preparation, and the accumulation of a new compound, which was not detected in non-elicited cultures, was observed. The accumulated compound was isolated and shown to be 2,5-dimethoxy-1,4-benzoquinone by 1H-NMR, 13C-NMR and electron ionization (EI) mass spectra. While it is well known that this compound shows antibacterial activity against Staphylococcus aureus, its presence in ginseng root has not been reported to date. Levels of the compound in the media increased rapidly, reaching a maximum level of 65.10 +/- 4.96 microg/g fresh weight at approximately 12 h after treatment with the yeast elicitor preparation. The maximal level of the compound in medium from the culture treated with an elicitor preparation from the culture broth of B. cinerea was 46.13 +/- 10.42 microg/g fresh weight after 24 h of incubation.     

真菌诱导子对茶条槭细胞没食子酸积累的影响

茶条槭（Acer ginnala Maxim.）叶片中含有没食子酸,但含量较低。真菌诱导子可以增加植物中一些次生代谢产物的含量,但其机理尚不十分清楚。本研究在茶条槭细胞悬浮培养的对数期加入内生真菌（Phomopsis sp.）诱导子,茶条槭细胞中没食子酸含量在24 h后开始增加,48 h时没食子酸含量达到峰值,最高含量为12.2 mg·g^-1 DW,是对照的1.58倍。茶条槭细胞对内生真菌诱导子的防御反应不同于对病原和非生物胁迫。真菌诱导子不提高培养液中pH值,也不明显增加胞内Ca²⁺浓度,但增大细胞膜通透性。培养液电导率差异显著,细胞核发生分裂,说明真菌诱导子可能促进茶条槭细胞核内有丝分裂,促使茶条槭细胞对培养液中的无机盐离子的吸收,以满足细胞生长的需要。PAL酶活性升高,在48 h时为对照的1.75倍,说明PAL酶可能参与了真菌诱导没食子酸的合成。