A Fluorescent Probe based on a Carbazole Derivative for Detecting Brilliant Blue in Food

Here a fluorescent probe based on a carbazole derivative(CNS)was developed to increase the detection range and reduce the detection limit of brilliant blue.Characteristics of CNS are studied.Due to the quenching ability of colorants,CNS shows an excellent current response to brilliant blue(from 1 to 10μM)with a detection limit of 2.7×10^(-8)mol/L(3σ/k)in the conditions of a 1:1 volume ratio of water to tetrahydrofuran.And the stability and reproducibility of CNS in the detection of actual samples indicate great potential for application.

Effects of Temperature on Determination of Protein Concentration with Coomassie Brilliant Blue Method

[Objective] This study aimed to investigate the effects of temperature on determination of protein concentration with Coomassie Brilliant Blue method,thus proving advice and guidance for accurate determination of protein concentration.[Method] With Coomassie Brilliant Blue method,the concentrations of different bovine serum albumin samples were determined under different temperatures and incubation time.[Result] According to the standard curve,when the determination range of protein concentration was 0-100 mg/ml,the determined protein concentration was relatively stable after incubation at 20 ℃ for 20-30 min.Furthermore,the determination result of higher protein concentration with Coomassie Brilliant Blue method was less affected by various factors.[Conclusion] In determination of protein concentration with Coomassie Brilliant Blue method,temperature,sample concentration and incubation time were important factors affecting the accuracy of experimental results.

Decolourization of Reactive Brilliant Blue KN-R by immobilized cells of Aspergillus ficuum

Aspergillus ficuum was immobilized with sodium alginate, and decolourization of Reactive Brilliant Blue KN-R was studied on immobilized and free Aspergillus ficuum. The optimal preparation condition of the strain immobilization was obtained by the orthogonal test, it is sodium alginate 3%, CaCl_2 5%, wet mycelia 30 g/L, calcific time 8 h. It was found that the immobilized cells could effectively decolourize Reactive Brilliant Blue KN-R, the optimum temperature and pH were 33℃ and 5.0, respectively. The kinetics study of decolourization of immobilized cells showed that the decolourization of Aspergillus ficuum immobilized conformed to zero-order reaction model. The decolourization efficiency of immobilized cell compared with that of free cell in different physical conditions. Results showed that the decolourization of immobilized cells with mycelia had the best efficiency. The immobilized cells could be reused after the first decolourization.

Brilliant blue G attenuates lipopolysaccharide-mediated microglial activation and inflammation

Previous studies have confirmed that oxidized adenosine triphosphate, a P2X7 receptor antagonist, attenuates lipopolysaccharide-mediated microglial activation and inflammatory expression following neuronal damage in rat brain. NaCI and temperature may affect the potency of oxidized adenosine triphosphate. Brilliant blue G is a derivative of a widely used food additive and has little toxicity. This study explored the effects of brilliant blue G, a selective P2X7 receptor antagonist, on microglial activation and inflammation. Results demonstrated that brilliant blue G inhibited the release of cydooxygenase-2 and interleukin-6 in BV2 cells. Immunofluorescence displayed that brilliant blue G could suppress lipopolysaccharide-induced microglial activation. This study used RNA interference to block P2X7 receptor expression and found that small interfering RNA also suppressed the release of cyclooxygenase-2 and interleukin-6 in BV2 cells. These results suggested that downregulation of the P2X7 receptor by brilliant blue G was involved in the inhibition of microglial activation and inflammation.

2DGE-coomassie brilliant blue staining used to differentiate pasteurized milk from reconstituted milk

Differentiating pasteurized milk and reconsti-tuted milk by scientific approach was necessary to defend consumer from economic fraud of wrong labeling. In this paper 2DGE (2 Dimen-sional Gel Electrophoresis)-coomassie brilliant blue staining method was employed and sig-nificant color intensity changing was observed among raw milk, pasteurized milk, UHT milk and reconstituted milk. For example, the intensity of 10 protein spots including casein and lac-toglobulin reduced more than two folds from pasteurized milk to reconstituted milk. However, DIGE (Differential Gel Electrophoresis) assay showed that the majority protein remained simi-lar level from pasteurized milk to reconstituted milk. Therefore the color fading of coomassie brilliant blue stained 2D gels may be due to other biochemical reaction, such as Maillard reaction, instead of protein degradation. Stability of 2DGE pattern was confirmed by running six gels of the same sample in parallel and software analysis showed that all proteins were at similar level. Two commercialized pasteurized milk samples and one reconstituted milk sample were tested by 2DGE-coomassie blue staining method and re-constituted milk could be easily identified.

An improved Coomassie Brilliant Blue (CBB R-250) staining to proteins in gels

An improved CBB staining with higher sensitivity than that of the typical CBB staining was reported.The main improvement was using a fixing step of 25% trichloroacetic acid(TCA) before CBB staining.For most proteins studied,the sensitivity of the improved CBB staining was about twice as high as that of the typical method.For basic and low molecular weight proteins such as ribosomal proteins,the sensitivity of this improved staining method was about 3.5-28 times that of the typical method.It was speculated that the improved procedure would be suitable for exact quantitative analysis of proteins fractionated by SDS-PAGE,especially for basic and low molecular weight proteins.On the other hand,this new modified method might be also applied to multidisciplinary studies,such as biological researches and nuclear sciences.

Fe-Mn-sepiolite as an effective heterogeneous Fenton-like catalyst for the decolorization of reactive brilliant blue

A study of the decolorization of reactive brilliant blue in an aqueous solution using Fe-Mn-sepiolite as a heterogeneous Fenton-like catalyst has been performed. The Fourier transform infrared （FTIR） spectra of the catalyst showed bending vibrations of the Fe-O. The Xray diffraction （XRD） patterns of the catalyst showed characteristic diffraction peaks of α-Fe203, γ-Fe203 and MnO. A four factor central composite design （CCD） coupled with response surface methodology （RSM） was applied to evaluate and optimize the important variables （catalyst addition, hydrogen peroxide dosage, initial pH value and initial dye concentration）. When the reaction conditions were catalyst dosage = 0.4 g, [H202]= 0.3 mL, pH= 2.5, [reactive brilliant blue]o = 50mg·L-1, and volume of solution = 500 mL at room temperature, the decolorization efficiency of reactive brilliant blue was 91.98% within 60min. Moreover, the Fe-Mn-sepiolite catalyst had good stability for the degradation of reactive brilliant blue even after six cycles. Leaching of iron ions （ 〈 0.4 mg·L-l） was observed. The decoloring process was reactive brilliant blue specific via a redox reaction. The benzene ring and naphthalene ring were first oxidized to open ring; these were then oxidized to the alcohol and carboxylic acid. The reactive brilliant blue was decom- posed mainly by the attack of .OH radicals including surface-bound .OH radicals generated on the catalyst surface.

Biodegradation and detoxification of the triphenylmethane dye coomassie brilliant blue by the extracellular enzymes from mycelia of Lactarius deliciosus

Fungi play an important role in dying wastewater treatment.In this work,the mycelia of Lactarius deliciosus exhibited an excellent capacity in decolorizing coomassie brilliant blue(CBB).The results demonstrated that the mycelia could treat CBB with high concentrations over a broad range of pH and temperature.The decolorization rate of 99.19%and the removal rate of 16.31 mg·L^(‒1)·h were realized.The mycelia could be recycled from decolorizing process for 19 times,indicating a good re-usability.It verified that the lignin peroxidase(121.65 U·L^(‒1))and manganese peroxidase(36.77 U·L^(‒1))were involved in the degradation and decolorization process of CBB.Toxicity assessments indicated the seed germination rate was up to 82.22%while inhibition to Escherichia coli decreased dramatically and no significant effect on Caenorhabditis elegans growth was found.The removal of CBB was a synergistic process accomplished by adsorption and biodegradation.The mycelia could be used for eco-friendly CBB treatment.

Application of PDE3 and Brilliant Cresyl Blue in In-vitro Culture of Sheep Oocyte

[Objective] The aim of this study was to increase the viability of sheep oocytes in vitro by using phosphodiesterase type 3（PDE 3） inhibitor milrinone combined with brilliant cresyl blue（BCB） staining.[Method] The differences between BCB tested and morphologically selected oocytes,as well as the effect of them on embryo development were compared;and then suitable inhibitive time of milrinone to sheep oocytes in vitro was studied and used in BCB-oocytes for in vitro embryo production（IVEP）.[Result] The BCB＋ oocytes percentage in A-and B-level sheep oocytes was 64.42%,which was extremely significantly higher than that in C-level（17.0%）.The maturing rate,cleavage rate and blastocyst rate of BCB＋ oocytes（86.16%,85.29% and 34.40%） of was significantly higher than those of BCB-oocytes（50.94%,36.19% and 6.73%）.The best time for PDE 3 inhibitor delaying the sheep oocyte mature in vitro was 6 h.In addition,the rate of embryo development in vitro could be significantly increased by inhibiting the BCB-oocytes for 6 h with Milrinone.[Conclusion] The study will provide reference for improving the efficiency of sheep oocytes culture in vitro.

Selection of oocytes for in vitro maturation by brilliant cresyl blue staining： a study using the mouse model

Selecting oocytes that are most likely to develop is crucial for in vitro fertilization and animal cloning. Brilliant cresyl blue （BCB） staining has been used for oocyte selection in large animals, but its wider utility needs further evaluation. Mouse oocytes were divided into those stained （BCB＋） and those unstained （BCB-） according to their ooplasm BCB coloration. Chromatin configurations, cumulus cell apoptosis, cytoplasmic maturity and developmental competence were compared between the BCB＋ and BCB- oocytes. The effects of oocyte diameter, sexual maturity and gonadotropin stimulation on the competence of BCB＋ oocytes were also analyzed. In the large- and medium-size groups, BCB＋ oocytes were larger and showed more surrounded nucleoli （SN） chromatin configurations and higher frequencies of early atresia, and they also gained better cytoplasmic maturity （determined as the intracellular GSH level and pattern of mitochondrial distribution） and higher developmental potential after in vitro maturation （IVM） than the BCB-oocytes. Adult mice produced more BCB＋ oocytes with higher competence than the prepubertal mice when not primed with PMSG. PMSG priming increased both proportion and developmental potency of BCB＋ oocytes. The BCB＋ oocytes in the large-size group showed more SN chromatin configurations, better cytoplasmic maturity and higher developmental potential than their counterparts in the medium-size group. It is concluded that BCB staining can be used as an efficient method for oocyte selection, but that the competence of the BCB＋ oocytes may vary with oocyte diameter, animal sexual maturity and gonadotropin stimulation. Taken together, the series of criteria described here would allow for better choices in selecting oocytes for better development.

Voltammetric Determination of Heparin Based on Its Interaction with Brilliant Cresyl Blue

Heparin is a polysaccharide of glycosaminoglycan class, which consists of repeating disaccharide units of iduronic/glucuronic acid and glucosamine residues with many biological functions. Many methods have been proposed for the detection of heparin, including UV-Vis spectrophotometry, the light scattering technique, HPLC and electro phoresis and flow injection analysis, etc.. But there are few reports about the detection of heparin by means of an electrochemical method. Electroanalytical methods are useful tools in bioanalytical chemistry because of their advantages, such as their instrumental simplicity, moderate cost and portability. The binding reactions of organic molecules with biomolecules such as DNA and proteins have been widely studied. In acidic solution, heparin is highly negatively charged due to the dissociation of the sulfate and carboxyl groups in its molecule, which can easily interact with cationic dyes. Based on this principle, in this work, a new electrochemical method for the determination of heparin was developed based on the interaction of heparin with brilliant cresyl blue（BCB）.

亮蓝G通过抑制P2X7/NLRP3通路减轻脑缺血再灌注大鼠神经炎症

目的:研究嘌呤受体P2X7在脑缺血再灌注损伤(CIRI)中的作用。方法:使用右侧大脑中动脉闭塞法(MCAO)制备大鼠CIRI模型,通过腹腔注射给予P2X7抑制剂亮蓝G(BBG)或NLRP3抑制剂MCC950处理。神经功能评分检测大鼠神经功能的改变,伊文思蓝染色检测血脑屏障完整性,通过酶联免疫吸附试验(ELISA)检测大鼠脑脊液中IL-1β和IL-18的含量,通过Western Blot检测右侧大脑皮质中P2X7、CD11b和NLRP3的表达。结果:BBG或者MCC950处理能改善CIRI大鼠神经功能,同时降低脑组织中伊文思蓝的含量,并降低脑脊液中IL-1β和IL-18的水平。此外,BBG可以降低右侧大脑皮质中CD11b和NLRP3的表达,但是MCC950只能降低CD11b表达,对P2X7表达没有明显影响。结论:BBG通过抑制P2X7/NLRP3通路减轻CIRI大鼠神经炎症。

Non-decoloured In-gel Digestion of Coomassie Blue-stained Proteins

A simplified method is presented for tryptic digestion of Coomassie brilliant blue(CBB)-stained proteins in polyacrylamide gels. Compared with conventional methods, the proposed method does not require a removal of the dye before digestion, and is thus faster and saves a lot of labor. The resulted digest can be analyzed by either RPLC/ESIMS or MALDI MS for identification of the protein in a conventional way. Model studies with bovine serum albumin(BSA) showed that 50 ng of the protein could be routinely identified. The simplified procedure displays a tendency to produce more incompletely cleaved peptides, which is favorable for improving the sequence coverage.

低电荷柱撑蒙脱土对考马斯亮蓝的吸附性能研究

采用微波法制得低电荷锂化蒙脱土(the reduced-charge lithiated bentonite,RCBT),再制备羟基铝柱撑剂,插层于RCBT中制备低电荷铝柱撑蒙脱土(the aluminum-pillared bentonite,Al/RCBT)。对Al/RCBT进行结构和形貌表征并考察它对考马斯亮蓝的吸附性能。研究表明:羟基铝柱撑剂成功插入RCBT层间,使蒙脱土的层间距增大了0.78 nm;最佳吸附pH值为2,吸附30 mg/L考马斯亮蓝溶液40 min即达到平衡,吸附容量达17 mg/g;Al/RCBT对考马斯亮蓝的吸附符合准二级动力学模型和Freundlich等温模型。

Ti/CoWO_(4)光阳极的制备及其光电催化性能

采用一步水热法在钛基底上制备一种具有优秀半导体特性的Ti/CoWO_(4)光阳极,通过改变水热反应时间可调节附着在基底表面的CoWO_(4)纳米球的数量,其中Ti/CoWO_(4)-6 h具有更大的活性面积、更高的电荷转移能力及更高的中间活性物种(自由基)生成效率.通过紫外可见(UV-Vis)光谱和扫描电子显微镜(SEM)等方式对材料进行表征,考察Ti/CoWO_(4)光阳极对活性艳蓝(KN-R)的光电催化(PEC)降解活性.结果表明,在PEC条件下,Ti/CoWO_(4)-6 h对KN-R(60 mg/L)脱色率可达84.97%,5次循环后降解率仍能达到74.91%.

煤气化细渣特性及其对不同染料的吸附性

为了研究煤气化细渣(coal gasification fine slag,CGFS)对不同性质染料的吸附性能,利用红外光谱分析(FTIR)、X射线衍射(XRD)、N2吸附-脱附和热重-差示扫描量热(TG-DSC)对CGFS表面官能团、物相组成、孔结构及热稳定性进行测试表征,通过染料吸附实验,研究CGFS对不同染料的吸附动力学和吸附热力学。结果表明:CGFS主要以无机矿物形式存在,主要晶相为SiO_(2),且碳含量较高,在550℃以下具有良好的热稳定性;CGFS对分散深蓝H-GL(DDB)几乎没有吸附效果;100℃干燥后的CGFS,在投加量0.1 g、环境温度25℃、吸附时间105 min、染料质量浓度50 mg·L^(-1)的条件下,对罗丹明B(RhB)及活性艳橙K-GN(RBO)的吸附量分别为48.62 mg·g^(-1)和46.03 mg·g^(-1)。CGFS对罗丹明B及活性艳橙K-GN的吸附过程均遵循拟一级动力学模型,不同温度下的等温吸附模型均符合Freundlich等温式。CGFS对罗丹明B和活性艳橙K-GN的吸附为物理吸附,平均吸附能分别为7.8326 kJ·mol^(-1)和2.4864 kJ·mol^(-1)。CGFS对2种染料的吸附过程都是吸热的,升高温度有利于染料的吸附。

考马斯亮蓝法测定果汁中蛋白质的含量

采用考马斯亮蓝法,对不同果汁中的蛋白质含量进行了测定。结果表明:蛋白质浓度在10-80μg/mL内与吸光度有良好的线性关系(R2=0.9964);样品平均回收率(n=3)分别为99.2%、98.8%、101.8%,RSD分别为0.64%、0.81%和0.58%(n=3)。该方法具有快速、灵敏度高、重现性好等特点。

微波辐射处理活性艳蓝KN-R染料溶液的研究

在活性炭存在下微波照射能使活性艳蓝KN R溶液迅速脱色 ,每g活性炭处理浓度为 30 0mg L的活性艳蓝KN R溶液5 0mL ,微波辐射 4min脱色率达 97 1% .

考马斯亮蓝法测定苹果组织微量可溶性蛋白含量的条件优化

以红星苹果果肉为试材,探讨不同提取缓冲液(磷酸缓冲液、Tris-HCl缓冲液和水)、缓冲液pH值、浓度、外源添加物和料液比等因素对苹果果肉可溶性蛋白提取效率的影响。结果表明:外源添加PVP和EDTA以及料液比是苹果可溶性蛋白提取率的主要影响因素。实验最终确定的提取条件为0.1mol/L pH9.0 Tris-HCl提取缓冲液(内含1mmol/L EDTA和1%PVP)、料液比1:25,此条件下苹果果实可溶性蛋白的有效测定含量为0.544%,为水提组(0.073%)的7.45倍。

考马斯亮蓝法测定野木瓜多糖中蛋白质的含量

采用考马斯亮蓝染色法对野木瓜多糖中蛋白质含量进行测定,在波长595 nm处测定吸光度,实验表明标准蛋白质在1.67μg/mL￣16.67μg/mL之间呈现良好的线性关系,该法简便迅速,灵敏度高、重现性好,是测定野木瓜多糖中蛋白质含量的有效方法,并通过此法测得野木瓜多糖中蛋白质平均含量为12.17%。