Penicillium and patulin distribution in pears contaminated with Penicillium expansum. Determination of patulin in pears by UHPLC-MS/MS

The danger of mycotoxin contamination entering the food supply through post-harvest infection is of perennial concern to food safety experts. To explore the distribution of Penicillium expansum and diffusion of its mycotoxin, patulin, in blue mold-damaged pears, Pyrus bretschneideri Rehd. cv. Yali obtained from markets and orchards in China were artificially inoculated with P. expansum and assayed for patulin accumulation and degree of fungal colonization. The inoculated pears were incubated until the lesions were 5, 10, 20, or 30 mm in diameter. We sampled tissue at a range of distances from the lesion, measured the spread of Penicillium by plate colony-counting methods, and used UHPLC-MS/MS to detect and quantify the patulin concentration. More P. expansum colony-forming units were isolated from pears with a higher degree of decay. Farther from the lesion, the fewer P. expansum colonies were observed, and the lower the patulin content detected. We found a significant difference in the patulin content between samples due to lesion size, and also in tissue sampled 10 mm away from the lesion. In consideration of this finding, to ensure food safety, we recommend that when a blue mold rot lesion on pear is 5, 10, or 20 mm in diameter, 20, 30, and 40 mm beyond the lesion should be removed, respectively. If a lesion surpasses 30 mm in diameter, the whole pear should be thrown away.

Detection of Patulin in Dairy Products by ELISA

The content of patulin in dairy products was detected by rapid ELISA assay. The pretreatment of samples was simple, with wide range of application. The standard product showed good linear relationship with the range of 0-5.4 μg/kg, and the linear relationship reached 0.999 3, with high sensitivity. It took shorter time, with a total time-consumption of 1 h. Moreover, it had good repeatability for analytical requirements.

Reduction of Patulin Content in Apple Juice Using Activated Carbone

The mycotoxin, patulin （4-hydroxy-4H-furo [3, 2c] pyran-2 [6H]-one）, is produced by a number of fungi common to fruit and vegetable-based products, most notably apples. Patulin contamination within apple products poses a serious health risk to consumers. Studies done on laboratory animals have demonstrated that patulin has a broad spectrum of toxicity, including mutagen city and carcinogenicity. The aim of the experiment was studying influence of selectively acting activated carbon powder--Ercarbon SH （Erbsloh, Germany） which is special produced for lowering HMF （hydroxy methyl furfural）, on reduction of patulin content in clear apple juice. Industrial apple row material with some damaged parts was pressed, juice was pasteurized at 95 ℃ during 2 min. After cooling on 55 ℃, enzymatic treated and clarified juice were filtered by 0.45 [am pore sizes membrane filter, Apple clear juice sample was divided for five parts. The samples of apple juice were diluted to 11.5° Brix and contacted with concentrations of 2, 2.5, 3 and 3.5 g/L activated carbon powder for 30 min. After filtration in the experimental samples, putulin was quantitatively determined by HPLC （high performance liquid chromatography with UV） detector at 276 nm. The research revealed that the best results were achieved by treatment with activated carbon in its powder form at concentration of 2.5 g/L with 30 min contact time.

Assessment of Patulin Content in Apple Puree and Apple and Fruit Puree by High Performance Liquid Chromatography

An analytical method was developed and validated for determination of patulin in apple puree by HPLC. Extraction and clean-up ofpatulin from clear extract are achieved on AFFINIMIP SPEPATULIN cartridges. Patulin is then separated on a Hypersil GOLD column 150 mm × 4 mm, 5 μtmand detected at 276 nm. The recovery in the range of 5 μg/kg-80 μg/kg was 81.47%. The limit of detection （LOD） was 1.36 μg/kg, and the limit of quantification （LOQ） was 4.55 μg/kg. The patulin content of the commercial samples of apple puree and samples of apple and fruit puree forinfants and young children as well as the samples of apple puree prepared from two apple varieties intended for processing （Jonathan, Florina） and obtained from conventional and uncertified organic cultures has been evaluated in this paper. The 44.83% patulin concentration of the analyzed samples were under the maximum level of the European Commission Regulation （EC） 1881/2006, in 46.55% of the analyzed samples patulin was not detected and in 8.62% of samples patulin concentration was lower than LOQ （European Comission, 2006a） Patulin was not detected in samples of apple puree intended for infants and young children consumption.

干酪乳杆菌清除苹果汁展青霉素对苹果汁品质的影响

目的:本课题组前期筛选到一株可以高效清除苹果汁中展青霉素的干酪乳杆菌Lactobacillus casei YZU01。本文主要研究L.casei YZU01清除苹果汁展青霉素过程中对苹果汁品质的影响。方法:以未添加和添加展青霉素的苹果汁作为对照,分别利用高效液相色谱法、p H计检测法、紫外分光光度法、比色法检测L.casei YZU01降解苹果汁展青霉素过程中苹果汁的有机酸(柠檬酸、酒石酸、富马酸、乙酸和L-苹果酸)和糖含量(葡萄糖和半乳糖)、酸度、非酶褐变指数和透光率、色度等苹果风味和品质相关指标。结果:L.casei YZU01清除苹果汁展青霉素过程中,苹果汁柠檬酸、酒石酸、富马酸和乙酸的含量增多,L-苹果酸、葡萄糖和半乳糖的含量减少,柠檬酸含量从0.18 g/kg上升至2.11 g/kg,酒石酸含量从2.3 g/kg上升至3.4 g/kg,富马酸含量从0.12 g/kg上升至0.15 g/kg,乙酸含量从0.00 g/kg上升至0.66 g/kg,L-苹果酸含量从7.31 g/kg下降至5.26 g/kg,葡萄糖含量从38.59 g/kg下降至1.59 g/kg,半乳糖含量从67.55 g/kg下降至28.37 g/kg。尽管干酪乳杆菌处理后苹果汁糖酸含量发生变化,但苹果汁酸度变化不大。干酪乳杆菌在清除展青霉素的过程中不会引起非酶促褐变反应,不会对色泽产生不良影响,但是会引起透光率的波动。在降解72 h后,干酪乳杆菌对苹果汁色度指标L^(*)值、b^(*)值的影响很小,而使a^(*)值稍稍增大,代表苹果汁绿色变浅。综上所述,干酪乳杆菌清除展青霉素的过程中对苹果汁糖和酸含量产生一定的影响,不会产生非酶褐变反应,对苹果汁色度影响较小。

食品中展青霉素的预防与减除技术研究进展

展青霉素主要是由青霉属、曲霉属、丝衣霉属等真菌产生的毒性极强的聚酮类次级代谢物,其中扩展青霉是其主要产毒菌。由于展青霉素具有水溶性、酸稳定性和耐热性而常出现在苹果、桃、梨、葡萄等水果、水果制品(果酒、果泥、果汁等)、蔬菜和谷物中,尤其是霉烂的苹果中展青霉素残留量很大,难以去除。需要采取适当的方法对产品中的展青霉素进行防治和控制,目前常见的物理、化学和生物方法虽然能够缓解展青霉素的污染问题,但是仍然存在一定局限性,如物理化学材料的安全评估不足和环境污染、潜在的二次污染、生防效力不足等问题。因此,探讨展青霉素防治和解毒方法的研究进展以及霉菌毒素防治的创新策略是很有必要的。本文综述用于控制食品中展青霉素含量的方法和有关机制,并讨论总结霉菌毒素防治可能的未来趋势,为解决食品中展青霉素污染问题提供理论参考价值。

光催化降解展青霉素的研究进展

展青霉素是由曲霉属和青霉属的某些真菌在特定条件下产生的有毒次级代谢产物,对人和动物具有急性毒性、生殖毒性、免疫毒性等。展青霉素易溶于水、在酸性介质中稳定存在。水果在生长、采收、贮藏和加工阶段均易受到展青霉素的侵染,因此为降低展青霉素带来的危害,保障人体健康,减少行业经济损失,研究安全高效的展青霉素降解方法十分必要。光催化降解技术因其具有高降解率、环境友好等优点,逐渐成为降解水果及其制品中展青霉素的研究热点。该文系统介绍了展青霉素的理化性质、生物合成、污染现状、危害及防控手段,重点阐述了光催化法及其降解展青霉素的机理和研究进展,提出了光催化降解展青霉素技术实现工业化应用的未来展望。

基于适配体检测水果及其制品中棒曲霉素的研究进展

棒曲霉素是广泛分布于各种水果、谷物及农产品中的一种真菌毒素,在较低浓度下产生持久性的毒性作用,对人类和动物健康造成严重的危害。随着人们对食品安全关注度的增加,棒曲霉素在水果及其制品中快速检测方法的研究引发广泛关注。适配体传感器因灵敏度高、耗时短、易操作及开发成本低等优点,在毒素快速检测方面具有潜在的开发和应用优势。本综述从棒曲霉素适配体筛选入手,着重介绍了基于电化学、光学和光电化学原理的适配体传感器在检测毒素中的原理、策略和应用,并展开分析其当前的发展现状、局限性和未来发展前景,旨在对水果及其制品中棒曲霉素有效检测和风险评估提供有益的见解,为棒曲霉素快速检测方法的研究和发展提供一定参考。

腐烂阿克苏红富士苹果中毒素的检测方法与迁移规律的研究

为了明确腐烂苹果中的6种真菌毒素的含量及其迁移规律。采用超高效液相色谱-质谱技术(UPLC-MS/MS)结合超高效液相色谱(HPLC),通过对腐烂的阿克苏红富士苹果中交链孢酚-AOH(Alternariol)、交链孢酚单甲醚-AME(Alternariol monamethyl ether)、细交链格孢酮酸-TEA(Tenuazonic acid)、交链孢烯-ALT(Altenuene)、腾毒素-TEN(Tentoxin)、展青霉素-PAT(Patulin)6种毒素的产毒范围、产毒条件、检测方法及迁移规律等方面进行了相关研究。结果表明,交链孢毒素广泛存在于霉变的苹果中,且随着贮藏时间的延长毒素不断累积;扩展青霉产生展青霉素的最适温度为20~25℃,且随着培养时间的延长,产毒量呈现增加的单峰性变化趋势,同时高湿条件有利于展青霉素的产生。

Patulin Imprinted Nanoparticles Decorated Surface Plasmon Resonance Chips for Patulin Detection

In this study,the patulin imprinted and the non-imprinted nanoparticles are synthesized by the two-phase mini emulsion polymerization method and characterized by zeta-size analysis,Fourier transform infrared spectroscopy,and scanning electron microscopy.Afterwards,the patulin imprinted and the non-imprinted nanoparticles are attached on the surface of surface plasmon resonance(SPR)chips.The patulin imprinted and the non-imprinted SPR nanosensors are characterized by using atomic force microscope,ellipsometer,and contact angle measurements.Kinetic studies for patulin detection are carried out in the concentration range of 0.5nmol-750nmol.The limit of detection and the limit of quantification values are obtained as 0.011 nmol and 0.036 nmol,respectively.In all kinetic analysis,the response time is 13 min for equilibration,adsorption,and desorption cycles.The selectivity studies of the patulin imprinted and the non-imprinted SPR nanosensors are determined in the presence of ochratoxin A and aflatoxin Bl.In order to demonstrate the applicability,validation studies of the patulin imprinted SPR nanosensor are performed by liquid chromatography-tandem mass spectrometry(LC-MS).

发酵和浸泡工艺对山楂酒安全指标的影响

为了探究不同浸泡比例和酿造工艺对山楂酒品质的影响,比较了浸泡山楂酒、发酵山楂酒两种工艺对山楂酒中氰化物、氨基甲酸乙酯、展青霉素等食品安全关键指标的影响。结果发现,随着山楂用量的增加,浸泡酒中氰化物含量增加,EC含量降低,但与原料间无比例关系。而山楂发酵酒中氰化物含量为0.078 mg/L,略高于浸泡酒,未检出EC。浸泡山楂酒和发酵山楂酒的氰化物和氨基甲酸乙酯均不超限量标准,制约山楂酒品质的主要因素是展青霉素。发酵山楂酒中展青霉素的含量高达109.17μg/kg,远超国家限量标准,而浸泡酒中仅为29.74~37.47μg/kg。综合安全指标,浸泡法制备的山楂酒更安全,并且浸泡比例为1∶1时其口感和风味更佳。采用发酵法制备山楂酒时,建议在发酵之前,先去除或钝化山楂果实上面的展青霉素生产菌,以杜绝展青霉素的产生。

卡利比克迈耶氏酵母对水果采后病害的抑制及对展青霉素的降解机制

为了明确拮抗酵母卡利比克迈耶氏酵母Meyerozyma caribbica对果实采后病害的抑制效果及其对毒素的降解机制,本文研究了卡利比克迈耶氏酵母结合辅助因子褐藻寡糖(alginate oligosaccharide,AOS),对草莓、梨、苹果、番茄的青霉病、灰霉病和黑斑病的抑制效果,以及拮抗酵母不同处理液对展青霉素(patulin,PAT)体外降解的机制。结果表明,浓度为1×10^(8) cfu/mL的M.caribbica可有效抑制草莓、梨、苹果青霉病,草莓、番茄、葡萄灰霉病以及番茄、梨、葡萄黑斑病的发生,添加5 g/L的AOS能显著增强M.caribbica的抑制效果;M.caribbica发酵液可以有效降解苹果伤口处的PAT,处理后8 d其降解率为30.35%,经AOS诱导后,其对PAT的降解效率达到39.15%。体外条件下,接种M.caribbica后27 h可将10μg/mL的PAT完全降解;M.caribbica主要是通过活细胞代谢降解PAT,同时AOS可显著增加M.caribbica的降解能力,说明卡利比克迈耶氏酵母是一株生防潜力较好的菌株,本研究为该生防菌株的进一步应用奠定了基础。

低温等离子体对展青霉素脱毒研究进展

低温等离子体技术能有效分解水果中的展青霉素,作为一项新兴的杀菌去毒技术,不仅维持了食品的新鲜度,还有助于提升食品的感官特性以及功能性和营养价值。本文旨在推进一种取代传统化学去毒方法的新技术,以减少展青霉素对消费者健康的潜在威胁,确保食品安全。

石墨化碳黑净化柱结合HPLC-PDA和LC-MS/MS快速检测苹果汁中展青霉素

基于石墨化碳黑材料制备了一种固相萃取柱(GCB柱),结合高效液相色谱-二极管阵列检测法(HPLC-PDA)和液相色谱-串联质谱法(LC-MS/MS)评估了GCB柱和4种商业化固相萃取柱(Retain AX PAX、MAX和HLB)的净化效果,并对澄清型苹果汁中影响展青霉素准确定量的杂质进行了分析。结果发现,苹果汁经上述5种净化柱净化后,大大降低了杂质干扰,色谱图、信噪比和基质效应显著改善。其中,GCB净化为HPLC-PDA分析提供了理想的色谱图,为LC-MS/MS分析提供了可接受的基质效应(-14%)、优于HLB净化的色谱图以及与Retain AX净化相当的信噪比。建立的稳定同位素稀释-液相色谱-串联质谱法(SIDA-LC-MS/MS)可以克服基质效应和净化损失对检测结果准确性的影响。采用HPLC-PDA和SIDALC-MS/MS分析时,GCB净化比HLB净化的方法更灵敏;MAX、HLB和GCB净化均能得到较好的回收率(82%~102%)和较小的相对标准偏差(≤9%)。所开发的GCB净化方法仅需上样和洗脱2步,且在重力作用下过柱仅需10 min,比其他固相萃取净化更简单快捷,净化能力良好。实际样品经GCB柱净化和HPLC-PDA、SIDA-LC-MS/MS分别分析,展青霉素的平均含量为34μg·kg-1。GCB柱较好的净化效果和较低的使用成本将有助于其在展青霉素常规检测中的广泛应用。

棒曲霉素的毒性及其机制研究进展

棒曲霉素作为一种有毒的真菌次级代谢产物,广泛存在于果蔬、谷物、坚果等食品及中药材中,并可通过食物摄入、皮肤接触等方式进入机体,进而对人类和牲畜的健康造成严重威胁。棒曲霉素具有基因毒性、免疫毒性、生殖毒性等多种毒性,能够损伤机体的肠、肾、肝等器官组织;棒曲霉素的毒性机制包括诱导生物大分子结构损伤、诱导氧化应激损伤、诱导细胞自噬、破坏肠道菌群稳态等。本文介绍近年来棒曲霉素在食品中的污染情况,重点阐述棒曲霉素的毒性及其毒性机制的最新研究进展,旨在为棒曲霉素的解毒研究提供理论参考。

展青霉素免疫学检测方法研究进展

展青霉素(patulin,PAT)作为一种对人类和动物有致畸、致癌等多种危害的真菌毒素,极易污染水果、蔬菜和谷物及其制品等。鉴于PAT污染范围广、超标检出多等问题,针对该毒素的即时检测对保障食品安全至关重要。免疫分析是快速检测真菌毒素污染的有效手段之一。但是,尚未有灵敏性好、实用价值高的PAT单克隆抗体和基因工程抗体报道。本文综述了PAT免疫学检测方法研究现状,并通过梳理其免疫学检测发展历程,提出高效特异性PAT单克隆抗体制备的阻碍主要包括PAT存在较大的极性、非免疫原性、在动物体内易被降解的特性及抗体制备选用的类似物结构偏差过大等。因此,本文认为筛选或制备结构稳定且更接近PAT的类似化合物可能是特异性PAT抗体制备的关键。另一方面,随着新型材料和技术(如电化学传感器)的发展,应用性能优良的抗体替代物建立新型免疫学或非免疫学检测方法的前景非常广阔,本文为PAT快速免疫检测方法的建立和应用提供理论依据和参考。

辉光放电等离子体(GDP)对苹果汁中棒曲霉素(PAT)降解效果及对风味物质的影响

棒曲霉素(PAT)是苹果汁中最常见的真菌毒素,对消费者健康和经济发展有很大危害,本文研究了辉光放电等离子体(Glow discharge plasma,GDP)对苹果汁中PAT的降解作用及对苹果汁风味物质的保护作用。结果表明:当直流电压为550 V、电流范围为10~90 mA时,GDP处理苹果汁15 min时PAT降解率达到92.89%,在30 min内,可溶性固形物和酚类物质无明显变化,电导率、氧化还原电位、色值略升高,pH略有降低;20 min后利用气相色谱质谱联用仪(Gas chromatography and mass spectrometry,GC-MS)可在苹果汁中检测出38种风味物质,其中包括酯类8种,醇类7种,醛酮类20种和3种其他类,且比原苹果汁增加了苯乙酮和6,10-二甲基-5,9-十一双烯-2-酮,前者具有似甜香味,后者具有香精油的味道,使苹果汁味道更加鲜美。该研究结果可为GDP降解苹果汁中PAT和对苹果汁风味物质的保护作用提供依据。

二氧化钛/石墨氮化碳复合材料对棒曲霉素的吸附与光催化降解作用研究

目的探究二氧化钛/石墨氮化碳(titanium dioxid/graphite carbon nitride,TiO_(2)/g-C_(3)N_(4))复合材料对棒曲霉素(patulin,PAT)的吸附与光催化降解作用。方法通过超声混合后再煅烧的方法制备TiO_(2)和g-C_(3)N_(4)的复合材料(TiO_(2)/g-C_(3)N_(4))。分别使用傅里叶转换红外光谱分析仪(Fourier transform infrared spectrometer,FTIR)和比表面及孔径分析仪(specific surface and aperture analyzer,BET)对3种材料进行测试分析,并研究单一材料与复合材料分别对PAT的吸附作用、复合材料在可见光下的光催化效果及暗吸附与光降解之间的协同作用。结果TiO_(2)/g-C_(3)N_(4)复合材料的FTIR图中出现了TiO_(2)的特征峰O-H基团和Ti-O、g-C_(3)N_(4)的特征峰C=N和CN,表明成功合成了TiO_(2)/g-C_(3)N_(4)复合材料。结果表明TiO_(2)和g-C_(3)N_(4)复合后的吸附及光催化降解效果明显优于单一材料,且TiO_(2)/g-C_(3)N_(4)复合材料暗吸附与光降解之间存在协同作用,在温度为30℃、复合材料添加量为10 mg、吸附时间3 min、光照时间5 min时,可完全降解初始质量浓度为0.5μg/mL的PAT。此外,TiO_(2)/g-C_(3)N_(4)对PAT的吸附存在多分子层化学吸附,且过程符合准二级动力学模型,对PAT的光催化降解过程符合准一级动力学模型。结论该复合材料可快速、高效地去除PAT,因此在果蔬及其制品、谷物和饲料中PAT的去除方面有较好的应用前景。

基于免疫脂质体的荧光分析法检测棒曲霉素

棒曲霉素是一种霉菌产生的天然毒素,曲霉菌、丝衣霉菌、青霉菌、毛霉和根霉等真菌均可产生,能污染水果、蔬菜、谷物和奶酪等多种食物,对食品安全造成威胁。传统的棒曲霉素检测方法需用有机溶液进行分离和浓缩,对环境产生一定的压力。针对传统方法的缺陷,本文利用兔抗棒曲霉抗体及其修饰的脂质体开发一种快速、灵敏、环境友好的荧光检测方法,检测限可达8μg/L,低于欧洲婴儿和幼儿食品监管要求(10μg/L)。本方法快速、灵敏、环境友好,可用于苹果汁等食品中棒曲霉毒素的检测。

固相萃取-超高效液相色谱-串联质谱法测定婴幼儿罐装辅助食品果泥中展青霉素的含量

提出了固相萃取-超高效液相色谱-串联质谱法测定婴幼儿罐装辅助食品果泥中展青霉素含量的方法。果泥样品经果胶酶酶解、乙酸乙酯提取后,经MAX固相萃取柱净化,浓缩复溶后采用Waters BEH C_(18)色谱柱分离,电喷雾离子源负离子和多反应监测模式下进行测定,同位素内标法定量。结果表明,展青霉素标准曲线的线性范围为10.0~200μg·L^(-1),检出限(3S/N)为2μg·kg^(-1)。按标准加入法进行回收试验,回收率为101%~112%,测定值的相对标准偏差(n=6)均小于4.0%。该方法应用于33份市售的婴幼儿罐装辅助食品果泥样品中展青霉素的测定,均未检出。