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1.
红曲的药用价值和保健功能日益引人关注,然而红曲中桔霉素的存在严重制约着红曲产品的开发,如何降低红曲桔霉素的含量是一个迫切需要解决的问题。本文概述了红曲桔霉素的毒性、生物合成途径及相关标准。并结合国内外研究进展,从发酵工艺,诱变育种,基因工程三个层面阐述了控制红曲桔霉素产生的对策,并对桔霉素今后的研究方向进行了展望。  相似文献   

2.
红曲霉桔霉素的检测方法及红曲霉产桔霉素的判别方法*   总被引:13,自引:0,他引:13  
建立了红曲霉真菌毒素桔霉素的HPLC检测方法。用谷氨酸和葡萄糖为唯一氮、碳源的培养基(MSG)液态摇瓶培养及红曲米固态培养,对30多株红曲霉产桔霉素的情况进行了普查,发现大多数红曲霉菌种可产生桔霉素。红曲霉的培养状态及条件对桔霉素的产生有重大影响。红曲霉菌种是否产桔霉素,可根据MSG培养基摇瓶发酵液中是否含有桔霉素来初步定性判断,为准确判断红曲霉菌是否产桔霉素,可采用多种培养法综合判断。  相似文献   

3.
Citrinin is one of the mycotoxins produced by Penicillium citrinum. We examined the decomposition products after heating citrinin in water at 140 degrees C and isolated a major product, citrinin H2 (3-(3,5-dihydroxy-2-methylphenyl)-2-formyloxy-butane). Citrinin H2 did not show significant cytotoxicity to HeLa cells up to a concentration of 200 microg/ml (% cytotoxicity: 39%) in 63 h of incubation, but citrinin showed severe toxicity at a concentration of 25 microg/ml (% cytotoxicity: 73%). HPLC analysis of citrinin after heating under various conditions indicates that citrinin H2 is mainly yielded from citrinin.  相似文献   

4.
红曲中桔霉素的检测及控制   总被引:1,自引:0,他引:1  
潘荣华  郑立忠  姜嘉善  蒙辉  徐小丽 《生物磁学》2013,(36):7160-7164,7134
红曲是指以大米为原料,用红曲菌属(Monascusspp.)红曲霉发酵培养制得,具有红色的颗粒或用其制成的粉末。目前红曲可分为色曲、酒曲和功能性红曲。在红曲霉的发酵过程中,同时与红曲色素相伴产生一种有害的次级代谢产物一桔霉素。研究表明桔霉素具有肾毒性,可致畸、致癌和诱发基因突变。桔霉素的存在,制约了红曲在食品及药品方面的广泛应用,在一定程度上阻碍了红曲产业的发展。为此,在红曲生产中如何快速准确检测桔霉素以及有效地防控桔霉素,是我们当前迫切需要解决的问题。本文对近年来国内外红曲中桔霉素的检测方法及控制策略进展进行了综述。目前,桔霉素的检测方法主要有抑菌圈法、TLC法、酶联免疫法和HPLC法等,其中HPLC法是检测红曲中桔霉素高效且应用最广泛的方法。桔霉素的控制主要从菌种选育,发酵工艺及产品后续处理等方面进行调控。目前尚没有成熟的控制策略全部去除桔霉素,只有采用低产桔霉素的菌种,适合的生产工艺及结合后续的物理或化学处理等综合措施,生产出符合桔霉素控制标准的高品质红曲产品。  相似文献   

5.
The ability of the mycotoxin citrinin to act as an inhibitor of iron-induced lipoperoxidation of biological membranes prompted us to determine whether it could act as an iron chelating agent, interfering with iron redox reactions or acting as a free radical scavenger. The addition of Fe3+ to citrinin rapidly produced a chromogen, indicating the formation of citrinin-Fe3+ complexes. An EPR study confirms that citrinin acts as a ligand of Fe3+, the complexation depending on the [Fe3+]:[citrinin] ratios. Effects of citrinin on the iron redox cycle were evaluated by oxygen consumption or the o-phenanthroline test. No effect on EDTA-Fe2+-->EDTA-Fe3+ oxidation was observed in the presence of citrinin, but the mycotoxin inhibited, in a dose-dependent manner, the oxidation of Fe2+ to Fe3+ by hydrogen peroxide. Reducing agents such as ascorbic acid and DTT reduced the Fe3+-citrinin complex, but DTT did not cause reduction of Fe3+-EDTA, indicating that the redox potentials of Fe3+-citrinin and Fe3+-EDTA are not the same. The Fe2+ formed from the reduction of Fe3+-citrinin by reducing agents was not rapidly reoxidized to Fe3+ by atmospheric oxygen. Citrinin has no radical scavenger ability as demonstrated by the absence of DPPH reduction. However, a reaction between citrinin and hydrogen peroxide was observed by UV spectrum changes of citrinin after incubation with hydrogen peroxide. It was also observed that citrinin did not induce direct or reductive mobilization of iron from ferritin. These results indicate that the protective effect on iron-induced lipid peroxidation by citrinin occurs due to the formation of a redox inactive Fe3+-citrinin complex, as well as from the reaction of citrinin and hydrogen peroxide.  相似文献   

6.
The stability of citrinin and deoxynivalenol during germination process of barley spiked with these mycotoxins at a level of 2/ig/g was investigated. Germinated barley was analyzed after 1, 3, and 5 days to follow the stability of citrinin and deoxynivalenol during the germination process. Two thin layer chromatographic methods were used for determinations of citrinin and deoxynivalenol. An average of 93.6% of citrinin and 77.1% of deoxynivalenol were destroyed within 5 days during the germination process of barley.  相似文献   

7.
Production and analysis of citrinin in corn.   总被引:5,自引:2,他引:3       下载免费PDF全文
A convenient method for the production and analysis of citrinin in corn is described. Up to 2.964 g of citrinin can be produced by Penicillium citrinum per kg of corn by harvesting on day 21 or later. The analysis method has a lower detection limit of 0.25 ppm. Heating citrinin-contaminated corn destroys citrinin but may produce another toxin instead.  相似文献   

8.
Wang C  Yang H  Chen M  Wang Y  Li F  Luo C  Zhao S  He D 《Biotechnology letters》2012,34(9):1745-1748
When Monascus MX was grown under blue light instead of in the dark, citrinin production increased from 478?mg?l(-1) to 698?mg?l(-1). To explain this, the expression of the pksCT gene, which encodes citrinin polyketide synthase, and of 5 ORFs around it, were monitored. Blue light enhanced citrinin production by upregulating the expression of orf1, orf3, and orf4, indicating that pksCT was not the key gene responsible for the quantity of citrinin production in blue light.  相似文献   

9.
Production of citrinin by various species ofMonascus   总被引:1,自引:0,他引:1  
Summary The production of citrinin by variousMonascus species was determinated using various culture mediums and conditions. The maximal production was obtained in fermentor usingM. ruber with concentrations of 380 mg/l. Since citrinin is a toxic product, it is essential that the production of red pigments as food additives fromMonascus sp. avoid the occurrence of citrinin; so, we argue that some nitrogen sources are unfavorable to the production of citrinin.  相似文献   

10.
Seven strains of Penicillium viridicatum isolated from country-cured ham produced citrinin in potato dextrose broth and on country-cured ham. None of the strains produced detectable amounts of citrinin at 10 C. The optimal temperature range for citrinin production was 25 to 30 C.  相似文献   

11.
红曲菌能产生多种有益的次级代谢产物,但红曲菌也产生一种对人和哺乳动物肝和肾有毒害的毒素,即桔霉素。因此控制毒素的产生是保障红曲产品安全性所必须的。故对桔霉素的合成途径及相关的基因做深入了解。6个桔霉素合成相关的基因成簇位于21 kb的DNA片段上。克隆了一个新基因(orf7基因),其位于该基因簇的外侧。采用基因敲除技术,构建红曲菌orf7基因缺失菌株。并采用紫外分光光度法检测orf7基因缺失菌株的红曲色素产量,HPLC法检测其桔霉素产量。orf7缺失菌株产红曲色素能力与出发菌株As3.4384相比没有变化;产桔霉素培养13~19 d,桔霉素的产量与出发菌株As3.4384相比增加了 142.4%。从而证实orf7基因与桔霉素代谢相关。  相似文献   

12.
1. The RNA synthesis of V79-E cells was inhibited by the mycotoxin citrinin time- and concentration-dependently. 2. Among the different RNA species mainly the rRNA synthesis was found to be inhibited by 200 microM citrinin. 3. At different precursor concentrations DNA synthesis was inhibited by citrinin after 30 min at least whereas labelling of the acid soluble fractions was found to be 3-fold higher than in untreated cells. 4. Remarkable perturbation of the DNA precursor metabolism, including release of precursor into the medium, was found to occur during citrinin treatment.  相似文献   

13.
The mycotoxins citrinin, patulin and terreic acid are absorbed by rice seedling roots and translocated to shoots. Ten day analysis of toxin treated plants showed persistence of citrinin, patulin and terreic acid. All three toxins at a concentration of 100 ppm showed phytotoxic activity indicating terreic acid in addition to citrinin and patulin as phytotoxins.  相似文献   

14.
Twenty-four isolates of Penicillium expansum Link from British Columbia (Canada) apples were cultured in yeast-extract sucrose (YES) at 25°C for 28 days to investigate production of patulin and citrinin. These isolates proved to be potent producers of citrinin, patulin, or in most cases, both mycotoxins. In every isolate, citrinin, patulin, or both compounds were produced at levels as high as 565 μg/mL (mean 269 μg/mL) and 100 μg/mL (mean 31 μg/mL), respectively. Of the 24 isolates, 4 produced citrinin only, and 2 produced patulin only. Overall, 83% of the isolates formed patulin and 91% formed citrinin. YES broth proved to be an effective medium for patulin and citrinin production. Other workers have noted that production of these mycotoxins in culture often presages production in fruits, so these results might help Canadian fruit processors evaluate and minimize mycotoxin levels in their products.  相似文献   

15.
The effects of mycotoxin citrinin on Ca2+ efflux and membrane permeabilization were studied in isolated rat liver mitochondria. The efflux rate observed when in presence of ruthenium red was higher when citrinin was added. Swelling experiments demonstrated Ca2+-dependent membrane permeabilization by citrinin. Catalase, butylhydroxitoluene (BHT), and dithiothreitol (DTT) did not protect swelling caused by Ca2+ plus citrinin. The protection conferred by ATP–Mg2+ and cyclosporin A in the latter experiments are strong indications of pore formation. These results suggest that citrinin can induce permeability transition by a mechanism that does not involve oxidative damage. © 1998 John Wiley & Sons, Inc. J Biochem Toxicol 12: 291–297, 1998  相似文献   

16.
Summary The degradation of citrinin by Penicillium citrinum in the presence of varying concentrations of glucose has been examined. Turnover of citrinin was found to be fast even in the presence of high concentrations of glucose. On the basis of these experiments, a role for citrinin in primary metabolism is postulated.  相似文献   

17.
The effects of citrinin on energy production along the respiratory chain and on glycolytic lactate production were examined in BHK-21 cultured cells. Citrinin inhibited the oxygen consumption rate by about 45 per cent. The respiratory rate of digitonin-treated cells energized with succinate, in the presence of ADP, was reduced by about 39 per cent. The mycotoxin inhibited the glucose utilization of BHK-21 cells by about 86 per cent. Cells treated with citrinin produced a small quantity of pyruvate, but were unable to produce lactate. It is concluded that BHK-21 cells cannot generate lactate when oxidative metabolism is inhibited by citrinin. The perturbations in BHK-21 cells caused by citrinin are due to alterations in mitochondrial function and in the glycolytic anaerobic pathway.  相似文献   

18.
The mycotoxin citrinin had antifungal activity under acidic conditions. At the minimum inhibitory concentration, it completely inhibited cellular respiration and partially inhibited the incorporation of radioactive precursors into macromolecules in Saccharomyces cerevisiae. It had no effect on cell permeability. In mitochondrial preparations, it significantly inhibited succinate oxidase and NADH oxidase. Rhizopus chinensis was more sensitive than S. cerevisiae; its growth and mycelial respiration at acidic pH were completely inhibited by lower concentrations of citrinin. The pH-dependent antifungal activity of citrinin seems to be associated with its uptake by fungi. Approximately half of the citrinin taken up was found in mitochondria. The main site of the antifungal action of citrinin, therefore, appears to be the mitochondrial electron transport system.  相似文献   

19.
A new rapid semi-quantitative fluorimetric assay for citrinin production testing in mould cultures has been developed. The chemical structure of the citrinin makes it a weak native fluorophore. This fluorescence can be strongly enhanced in an acidic environment. A standard curve where the concentration of HCl needed to show the yellow fluorescence signal of different concentrations of citrinin was established, thus providing a semi-quantitative method to prove the capacity of toxin production of fungal cultures. Two Penicillium strains from the Spanish National Collection of Type Cultures, were studied for the toxin production on YES broth at 25°C for 21 d. The culture was assayed daily for the presence/absence and quantification of citrinin by adding the HCl concentration set, and also quantified by RP-HPLC as a confirmation procedure. Experiments demonstrate that 5 d are necessary to show the presence of citrinin. As an illustration, a total of 48 strains of Penicillium isolated from cheese and cheese factories were analysed with the proposed method.  相似文献   

20.
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