An improved method for extraction of sorghum polymeric protein complexes

A method for fractionating sorghum proteins using extraction solvents and techniques designed to obtain polymeric protein structures (especially disulfide linked) was developed. Extraction and separation conditions were optimized in terms of completeness of protein extraction, sample stability, and analytical resolution. After pre-extraction of albumins and globulins, a 3-step sequential procedure involving no reducing agents was applied to ground whole sorghum flour. The three fractions obtained represented proportionally different protein polymer contents and molecular weight distribution as evidenced by comparative size exclusion chromatography. Protein composition also varied among the extracts with differences in kafirin composition and non-kafirin proteins detected in the fractions by RP-HPLC and SDS-PAGE analysis. The ability to quantify and further characterize sorghum polymeric protein complexes will be useful for additional studies linking protein structures with functionality and digestibility and variations for these properties within diverse sorghum germplasm.     

Effects of germination and kilning on the phenolic compounds and nutritional properties of quinoa (Chenopodium quinoa) and kiwicha (Amaranthus caudatus)

Quinoa (Chenopodium quinoa) and kiwicha (Amaranthus caudatus) are nutritious pseudocereals that originate from the Andean region. The aim of this research was to study the effect of germination and the subsequent kilning on the phenolic compounds and proximate composition in selected Peruvian varieties of quinoa (“Chullpi”) and kiwicha (“Oscar Blanco”). The germination process was carried out for 24, 48 and 72 h at 22 °C, and the kilning was performed with samples germinated for 72 h by drying the seeds at 90 °C for 5 min. Both processes increased the protein content of the samples. However, lipid content was reduced during germination. On the other hand, germination and kilning clearly increased the concentration of total phenolic compounds in both quinoa and kiwicha. Germination for 72 h either with or without kilning process resulted in a significant (p < 0.05) increase in the total content of phenolics compared to untreated materials, which was especially due to coumaric acid and a kaempferol tri-glycoside in quinoa and caffeoylquinic acid in kiwicha. Based on the results, germination and kilning may improve the nutritional quality of the Andean grains, encouraging the usage of the processed grains as ingredients in functional products for people with special gluten-free or vegetarian diets.     

Recent progress in analytical method development to ensure the safety of gluten-free foods for celiac disease patients

As laid down by the Codex Alimentarius, products bearing a gluten-free label must not contain gluten levels above 20 mg/kg to be safe for consumption by celiac disease patients. Analytical methods to detect gluten from wheat, rye and barley need to be sufficiently sensitive, specific, suitable for routine analyses and validated by collaborative studies. With continuous progress in the field of gluten analysis, the aim of this paper is to provide an up-to-date overview of legislation regarding gluten-free products worldwide, as well as immunochemical, proteomics-based, genomics-based and other methods designed to analyse gluten traces. While ELISA test kits and PCR are still most widely used in quality control, liquid chromatography tandem mass spectrometry (LC-MS/MS) is gaining more and more importance by providing unprecedented insights into gluten. Several other methods such as immunosensors, other sensors and microarrays are being developed. The pro's and con's of the different methods are discussed as well as the remaining challenges, including the need for improved extraction procedures, comprehensive reference materials and independent reference methods.     

香蕉中噻唑膦残留分析方法研究

建立香蕉中噻唑膦的超高效液相色谱串联质谱法(UPLC-MS/MS)残留测定方法。香蕉样品采用乙腈提取和PSA+C18分散固相萃取,采用UPLC-MS/MS多反应模式(MRM)进行分析测定。噻唑膦在添加水平0.01~1.0 mg/kg范围内,平均回收率为94.3%~107.5%,相对标准偏差为7.9%~11.0%。采用外标法定量,方法的检出限为0.001μg/m L,定量限为0.005 mg/kg。该方法简单、准确、重复性较好且节省溶剂,适用于香蕉中噻唑膦的残留检测。     

高密度二氧化碳对食品中蛋白质结构及其加工特性影响研究进展

非热加工技术已广泛应用于食品加工行业，高密度二氧化碳（dense phase carbon dioxide，DPCD）加工技 术作为一种新型的非热加工技术，因其无毒无害、能耗低、对食品品质影响小等特点，成为国内外食品加工技术研 究的焦点。蛋白质作为食品的重要组成成分，直接影响食品的风味、质构及营养。本文简要介绍DPCD加工技术概 况和特点，总结关于DPCD对蛋白质结构及加工特性影响和DPCD钝酶作用的最新研究进展，展望了DPCD加工技术 的发展前景，为今后非热加工技术应用于食品加工提供重要研究思路。     

SPI凝胶颗粒制备及其Pickering高内相乳液特性研究

制备了大豆分离蛋白（Soy protein isolate，SPI）凝胶颗粒，并使用该颗粒制备了稳定的Pickering高内相乳液。通过粒径和ζ 电位测定、冷冻扫描电镜和光学显微镜观察以及外观分析，以流变特性为指标，对SPI凝胶颗粒和Pickering高内相乳液特性进行研究。结果表明，SPI凝胶颗粒的粒径和ζ 电位随pH值的变化而变化，当SPI凝胶颗粒pH值为4.0～5.0时，临近SPI等电点，ζ 电位的绝对值最小，此时凝胶颗粒相互聚集，不能成功制备稳定的高内相乳液。在pH值为 9.0时，大豆分离蛋白凝胶颗粒紧密结合在一起，呈凝胶网络状结构。在碱性条件下，蛋白质质量分数为1.00%、内相体积分数为78%～82%时，可以制备稳定的Pickering高内相乳液。通过增加内相体积分数，使大豆分离蛋白凝胶颗粒稳定的Pickering乳液体系分布更加均匀，不易发生聚集，形成更加致密稳定的多孔结构，且具有更强的弹性凝胶乳液特性。     

基于单克隆抗体的O型口蹄疫病毒抗体固相竞争ELISA检测方法的建立

为建立评价O型口蹄疫病毒(FMDV)疫苗免疫水平的方法,本研究以单克隆抗体(MAb)3D9为捕获抗体,以HRP标记的MAb 8E8作为检测MAb,经过条件优化建立了基于MAb的检测O型FMDV抗体的固相竞争ELISA(SPCE)方法。对该方法进行了特异性、敏感性、重复性试验。结果显示,MAb 3D9的最佳稀释度为1:25 000,灭活O型FMDV抗原的最佳稀释浓度为1:3,HRP标记的MAb 8E8的最佳稀释度为15 000,当血清1:32稀释时,检测的临界值确定为45%。该方法分别检测A型FMDV抗体阳性参考血清以及牛冠状病毒、牛轮状病毒以及猪繁殖与呼吸障碍综合征病毒、猪圆环病毒、猪瘟病毒的标准阳性血清,检测结果均为阴性,未出现交叉反应。经检测,当阳性标准血清的抗体稀释度在1:512时,该方法仍具有较好的敏感性;批内和批间重复性试验的变异系数均小于10%,表明其重复性较好。并将该方法与液相阻断ELISA(LPBE)方法和病毒中和试验(VNT)的相关性进行了比较,结果显示该方法与LPBE和VNT的相关性分别为0.896和0.923。本研究为国内评价O型FMDV疫苗免疫水平建立了一种新的方法。     

混合沙粒对半开式叶轮离心泵磨损的影响

为了研究含有混合多种颗粒粒径的含沙水对离心泵过流部件磨损特性的影响,应用RNG k-ε湍流模型和SIMPLEC算法,基于颗粒离散相模型(DPM)和半经验的McLaury磨损模型,沙粒注入选用Rosin-Rammler分布的拟合方法,对一台半开式离心泵内固液两相流的磨损特性进行数值分析.研究结果表明:叶轮流道内沙粒组分中大颗粒有趋向叶片吸力面运动的趋势,当混合沙粒的粒径较小时,蜗壳内沙粒运动较为均匀,粒径越大,沙粒运动越贴近蜗壳壁面;不同粒径组分的沙粒在叶轮的压力面、吸力面和后盖板壁面上的平均停留时间分布相似,颗粒粒径越大,平均停留时间越小;在蜗壳壁面上沙粒组分中粒径不大于700 μm的沙粒平均停留时间分布规律与沙粒在叶轮过流壁面上的平均停留时间类似,大于700 μm的沙粒平均停留时间会随着粒径增加而增大;随着沙粒组分中大粒径沙粒的增加,叶片压力面的磨损强度逐渐减弱,叶片吸力面、后盖板和蜗壳的磨损强度逐渐增强.     

Use of serum amyloid A in equine medicine and surgery

Serum amyloid A (SAA) has become an indispensable part of the management of equine patients in general practice and specialized hospital settings. Although several proteins possess acute phase properties in horses, the usefulness of SAA exceeds that of other acute phase proteins. This is due to the highly desirable kinetics of the equine SAA response. SAA concentrations exhibit a rapid and pronounced increase in response to inflammation and a rapid decline after the resolution of inflammation. This facilitates the detection of inflammatory disease and real-time monitoring of inflammatory activity. SAA may be used in all stages of patient management: (1) before diagnosis (to rule in/rule out inflammatory disease), (2) at the time of diagnosis (to assess the severity of inflammation and assist in prognostication), and (3) after diagnosis (to monitor changes in inflammatory activity in response to therapy, with relapse of disease, or with infectious/inflammatory complications). By assessing other acute phase reactants in addition to SAA, clinicians can succinctly stage inflammation. White blood cell counts and serum iron concentration change within hours of an inflammatory insult, SAA within a day, and fibrinogen within 2–3 days; the interrelationship of these markers thus indicates the duration and activity of the inflammatory condition. Much research on the equine SAA response and clinical use has been conducted in the last decade. This is the prerequisite for the evidence-based use of this analyte. However, still today, most published studies involve a fairly low number of horses. To obtain solid evidence for use of SAA, future studies should be designed with larger sample sizes.