Comparativeassessmentofglycosylationofrecombinanthuman...(二)
Experimental sectionChemicals and reagentsOne lot of PuregonR-HP of 50 IU/0.5mL and two lots of PuregonR-HP of 100 IU/0.5mL (rhFSH) (Organon, Oss, Netherlands) were purchased in China. All strengths were presented as liquor. One lot of high purity uhFSH (>98%) was obtained directly from the manufacturer, Shanghai Techwell Biopharmaceutical Company (Shanghai, China), as active pharmaceutical ingredient. C......阅读全文
Comparative-assessment-of-glycosylation-of-recombinant-human-...(二)
Experimental sectionChemicals and reagentsOne lot of PuregonR-HP of 50 IU/0.5mL and two lots of PuregonR-HP of 100 IU/0.5mL (rhFSH) (Organon, Oss, N
Comparative-assessment-of-glycosylation-of-recombinant-human-...(四)
Site-specific characterization of N-glycans For intact N-glycopeptide analysis, chymotryptic digests of both hFSHs were subjected under UPLC equip
Comparative-assessment-of-glycosylation-of-recombinant-human-...(六)
(22) Wu, S. W.; Pu, T. H.; Viner, R.; Khoo, K. H. Novel LC-MS/MS product dependent parallel data acquisition function and data analysis workflow f
Comparative-assessment-of-glycosylation-of-recombinant-human-...(三)
LC-MS data processingN-glycan data were processed using UNIFI 1.7 with Glycobase 3+ (Waters Corporation, Milford, MA) for N-glycan structure. The pe
Comparative-assessment-of-glycosylation-of-recombinant-human-...(七)
Figure 3 MS2 spectra of 2-AB-labeled N-glycan structures. Diagnostic ions are marked with corresponding fragment structures. (a) NeuGc1NeuAc1HexNA
Comparative-assessment-of-glycosylation-of-recombinant-human-...(一)
Comparative assessment of glycosylation of recombinant human FSH and highly purified FSHHong Wang, Xi Chen, Xiaoxi Zhang, Wei Zhang, Yan Li, Hongrui Y
Comparative-assessment-of-glycosylation-of-recombinant-human-...(五)
Supporting Information(1) RP-UPLC-Q-TOF analysis of hFSHs subunits; (2) molecular weights and possible glycan structures of hFSHs subunits; (3) pr
Synthesis-of-Recombinant-Human-Cytokine-GMCSF-in-the--Seeds-of-Transge...
We are interested in studying plant systems as vehicles for the production of recombinant proteins of clinical relevance. There are a number of p
重组人表皮细胞生长因子(recombinant-human-EGF)
生物学功能:人表皮细胞生长因子(hEGF)不仅对上皮细胞而且对许多类型细胞均有促增殖作用,是与细胞的生长及分化有关的重要生长因子。hEGF具有多种生物活性,主要表现在:①在体内刺激皮肤组织、角膜和气管上皮组织的生长繁殖; ②加速角膜、皮肤等表皮创伤的修复; ③抑制胃酸分泌;④促进人皮肤上皮细胞、角膜
Comprehensive-identification-of-novel-proteins-and-Nglycosylation-sites二
ResultsIdentified novel royal jelly proteins To expand the number of known proteins in the RJ proteome, RJ proteins were extracted and digested wit
流式应用精选——微核检测(体内体外)
注:点击文章名称查看详情。文章名称样本仪器型号备注Assessment of the Genotoxic Potential of Azidothymidine in the Comet,Micronucleus, and Pig-a AssayBone Marrow and Peripheral
高通量测序技术在肠道菌群多样性研究中的应用(三)
一、饮食、能量摄取、肥胖与肠道菌群之间的关系:1. A core gut microbiome in obese and lean twins——2009《Nature》——if 36.102. An obesity-associated gut microbiome with increase
DNA重组技术(Recombinant-DNA)实验原理、用品和步骤(二)
【实验步骤】 1.PCR产物纯化 PCR产物经琼脂糖凝胶电泳,应用凝胶回收试剂盒回收纯化目的DNA片段。 2.目的DNA片段连接至T/A克隆载体 即重组DNA分子的构建 反应体系及条件如下: 3.转化 3.1 将感受态细胞置冰中融解。 3.2 将60μl感受态细胞移至无菌
In-vitro-Assessment-of-Metabolic--in-Suspension-Cryopreserved-Hepatocytes
实验概要BackgroundThe pharmaceutical and biotechnology industry’s goal is to discover therapeutic agents that are both safe and effective at treating or
CO2恒温摇床解决人胚肾-293-(HEK293)-细胞结团问题(一)
人胚肾 293 (HEK293) 细胞在重组蛋白表达中是最常见的宿主细胞。 这类细胞能够表达大量的膜蛋白,如 G 蛋白偶联受体 (GPCR) ,是无法在最常见的生物制药生产宿主,如:中国仓鼠卵巢 (CHO) 细胞中作表达。 HEK293 虽然是蛋白表达的极好宿主,然而 HEK293 细胞
Glycosylation-of-Antibody-Therapeutics:-Optimisation-for-Purpose
Recombinant antibody therapeutics represent a significant success story in terms of clinical benefit delivered and revenue (profit) generated wit
Assessment-of-Magnaporthe-grisea-mating-type-by-spore-PCR
Isolation of DNA from filamentous fungi for PCR analysis is usually time consuming and involves use of toxic chemicals such as phenol/chloroform. In S
Comprehensive-identification-of-novel-proteins-and-Nglycosylation-sites九
41. Schmidt O, Theopold U, Strand M: Innate immunity and its evasion and suppression by hymenopteran endoparasitoids. BioEssays 2001, 23(4):344–35
欧盟评估一种转基因大豆作为食品和饲料的安全性
2019年11月11日,欧盟食品安全局(EFSA)发布消息,欧盟食品安全局转基因生物小组(GMO Panel)评估了转基因大豆MON 87751×MON 87701×MON 87708×MON 89788用作食品和饲料的安全性。 经过评估,GMO小组得出结论,就对人类和动物健康以及环境的潜在影
Preparation-of-human-platelets
Preparation of human platelets 1. Human blood was taken from drug-free volunteers on the day of the experiment using acidic citrate dextrose
Production-of-Recombinant-Proteins-in-SuspensionCultured-Plant-Cells
Plants have emerged in the past decade as a suitable alternative to the current production systems for recombinant pharmaceutical proteins and, toda
Human-Embryonic-Stem-(ES)-Cell-Protocols——Freezing-Human-ES-Cells
Collagenase cells for approximately 7 minutes at 37 °C (until edges of colonies are curling up). With a 5 ml pipet, gently pipet and scrape colon
Human-Embryonic-Stem-(ES)-Cell-Protocols——Thawing-Human-ES-cells
Remove Human ES cells from liquid nitrogen storage tank. Fill out a freeze/thaw form.Thaw cryovial by gently swirling in waterbath until only a small
Steps-in-the-Glycosylation-of-Mammalian-Nlinked-Oligosaccarides
The biosynthesis pathway of N-glycans is a costly system with respect to the number of enzymes that are involved in the synthesis and trimming of N-gl
Human-Embryonic-Stem-(ES)-Cell-Protocols—Splitting-Human-ES-cells-onMatrige
based on splitting onto on plateWarm collagenase media to 37°C in a water bath.Aspirate media off of cell culture plate.Add the following amount of co
Human-Embryonic-Stem-(ES)-Cell-Protocols——Splitting-Human-ES-cells-on-MEFs
based on splitting onto one plateWarm collagenase IV split media to 37 °C in a water bath.Aspirate media off of cell culture plate.Add the following a
Characterization-and-Applications-of-PlantDerived-Recombinant-Antibodies
Expression of foreign proteins in plants has become a standard technique in plant molecular biology. Various plant species have been used to prod
Purification-of-recombinant-sBRF-M166L
Induction of BRF in bacteria and purification on Ni-NTA agaroseTransform BRF plasmid into strain BL21 DE3 (pLysS) or JM25 (DE3 containing the Arg tRNA
重组质粒(dna-recombinant-plasmid)的连接
质粒具有稳定可靠和操作简便的优点。如果要克隆较小的DNA 片段( <10kb) 且结构简单,质粒要比其它任何载体都要好。在质粒载体上进行克隆,从原理上说是很简单的,先用限制性内切酶切割质粒DNA 和目的DNA 片段,然后体外使两者相连接,再用所得到重组质粒转化细菌,即可完成。但在实际工作中,
Preparation-of-Sonicated-Human-DNA
Purpose:To break up high molecular weight human placental DNA into fragment sizes of 500 bp or less which can be used as competitor DNA in Southern an