Chanda Anindya, Roze Ludmila V, Pastor Alicia, Frame Melinda K, Linz John E
Department of Food Science and Human Nutrition, Michigan State University, East Lansing, Michigan 48824, USA.
J Microbiol Methods. 2009 Jul;78(1):28-33. doi: 10.1016/j.mimet.2009.03.014. Epub 2009 Apr 7.
Current studies in our laboratory demonstrate a functional link between vesicles, vacuoles and aflatoxin biosynthesis in the filamentous fungus, Aspergillus parasiticus. Under aflatoxin inducing conditions in liquid yeast-extract sucrose medium, A. parasiticus undergoes a shift from vacuole biogenesis to accumulation of an enhanced number of vesicles which exhibit significant heterogeneity in size and density. As a first step in conducting a detailed analysis of the role of these organelles in aflatoxin synthesis, we developed a novel method to purify the vesicle and vacuole fraction using protoplasts prepared from cells harvested during aflatoxin synthesis. The method includes the following steps: 1] preparation of protoplasts from mycelia grown for 36 h under aflatoxin inducing conditions; 2] release of vesicles and vacuoles from purified protoplasts in the presence of Triton X-100; and 3] fractionation of the vesicles and vacuoles using a "one-step high density cushion". The vesicle-vacuole fraction showed a 35 fold enrichment in alpha-mannosidase activity (vacuole marker) and non-detectable succinate dehydrogenase and lactate dehydrogenase activities (mitochondrial and cytoplasmic markers, respectively). Confocal laser scanning microscopy with the vacuole dyes MDY-64 and CMAC demonstrated that the fraction contained pure vesicles and vacuoles and was devoid of membranous debris. Transmission electron microscopy (TEM) confirmed that no mitochondria or unbroken protoplasts contaminated the purified fraction. The purified organelles exhibited significant size heterogeneity with a range of sizes similar to that observed in whole cells and protoplasts.
我们实验室目前的研究表明,在丝状真菌寄生曲霉中,囊泡、液泡与黄曲霉毒素生物合成之间存在功能联系。在液体酵母提取物蔗糖培养基中黄曲霉毒素诱导条件下,寄生曲霉经历了从液泡生物发生到大量囊泡积累的转变,这些囊泡在大小和密度上表现出显著的异质性。作为详细分析这些细胞器在黄曲霉毒素合成中作用的第一步,我们开发了一种新方法,利用从黄曲霉毒素合成期间收获的细胞制备的原生质体来纯化囊泡和液泡部分。该方法包括以下步骤:1] 在黄曲霉毒素诱导条件下培养36小时的菌丝体制备原生质体;2] 在Triton X - 100存在下从纯化的原生质体中释放囊泡和液泡;3] 使用“一步高密度垫层”对囊泡和液泡进行分级分离。囊泡 - 液泡部分的α - 甘露糖苷酶活性(液泡标记物)富集了35倍,而琥珀酸脱氢酶和乳酸脱氢酶活性(分别为线粒体和细胞质标记物)未检测到。用液泡染料MDY - 64和CMAC进行的共聚焦激光扫描显微镜观察表明,该部分含有纯净的囊泡和液泡,没有膜碎片。透射电子显微镜(TEM)证实纯化部分没有线粒体或未破碎的原生质体污染。纯化的细胞器表现出显著的大小异质性,其大小范围与在全细胞和原生质体中观察到的相似。