Endothelialwoundhealing(cellmigration)assay
DescriptionThis is a simple assay that can be used in any cell culture lab setup to test the effect of different compounds on endothelial cell migration. ProcedureGrow endothelial cells in complete media.Day 1: Trypsinize cells and add 4 x105 cells per well in a six well plate in complete media. After 8 h, change media to starvation media. Starve cells overnight in this media.Day 2:1) Remove media from cells.2) ......阅读全文
Isolation-of-human-corneal-endothelial-cells-(HCECs)
Isolation of HCECs1. The corneoscleral tissues were rinsed three times with primary cell culture system containing 50 mg/mL gentamicin and 1.25 mg
Isolation-and-cultivation-of-endothelial-progenitor-cells-(EPCs)
Circulating bone marrow (BM)–derived endothelial progenitor cells (EPCs) are recruited to the site of tissue regeneration and substantially contri
ex-vivo-expanded-endothelial-progenitor-cells
Cell Culture. 1. Total hPBMCs were isolated from blood of human volunteers by density gradient centrifugation. 2. Cells were plated on culture dishes
Keynote-Speaker:-Ying-Zeng
Ying Zeng Mr. Zeng is in charge of research and develop department of Lifotronic Technology Co., Ltd. IVD Division of Lifotronic has developed an el
AEBP1基因突变与药物因子介绍
这个基因编码羧肽酶A蛋白家族的一个成员。编码蛋白可能作为转录抑制因子发挥作用,并在脂肪生成和平滑肌细胞分化中发挥作用。对小鼠的研究表明,这种基因在伤口愈合和腹壁发育中起作用。该基因的过度表达与胶质母细胞瘤有关。This gene encodes a member of carboxypeptidas
与白血病相关的AEBP1基因编码功能描述
这个基因编码羧肽酶A蛋白家族的一个成员。编码蛋白可能作为转录抑制因子发挥作用,并在脂肪生成和平滑肌细胞分化中发挥作用。对小鼠的研究表明,这种基因在伤口愈合和腹壁发育中起作用。该基因的过度表达与胶质母细胞瘤有关。This gene encodes a member of carboxypeptidas
与黑色素瘤相关的AEBP1基因编码功能描述
这个基因编码羧肽酶A蛋白家族的一个成员。编码蛋白可能作为转录抑制因子发挥作用,并在脂肪生成和平滑肌细胞分化中发挥作用。对小鼠的研究表明,这种基因在伤口愈合和腹壁发育中起作用。该基因的过度表达与胶质母细胞瘤有关。This gene encodes a member of carboxypeptidas
AEBP1基因编码功能及结构描述
这个基因编码羧肽酶A蛋白家族的一个成员。编码蛋白可能作为转录抑制因子发挥作用,并在脂肪生成和平滑肌细胞分化中发挥作用。对小鼠的研究表明,这种基因在伤口愈合和腹壁发育中起作用。该基因的过度表达与胶质母细胞瘤有关。This gene encodes a member of carboxypeptidas
EPPK1基因突变与药物因子介绍
该基因编码的蛋白属于plakin蛋白家族,在细胞骨架结构的组织中起着重要作用这个家族成员由几个高度同源的plakin重复序列组成它可能维持上皮细胞角蛋白中间丝网络的完整性对小鼠原代蛋白的研究表明,它在伤口愈合过程中加速了角质形成细胞的迁移[由RefSeq提供,2013年10月]The protein
EPPK1基因编码功能及结构描述
该基因编码的蛋白属于plakin蛋白家族,在细胞骨架结构的组织中起着重要作用这个家族成员由几个高度同源的plakin重复序列组成它可能维持上皮细胞角蛋白中间丝网络的完整性对小鼠原代蛋白的研究表明,它在伤口愈合过程中加速了角质形成细胞的迁移[由RefSeq提供,2013年10月]The protein
Isolation-and-culture-of-rat-coronary-microvascular-endothelial-cells
CMVE were isolated from Wistar rat hearts by digestion of primary cell isolation kit.1. Hearts mounted on a Langendorff apparatus were perfused at 3
Actin-Capture-Assay
David AmbergDialyze purified GST fusion proteins and actin into PBS + 1mM MgCl2 .Mix 5ug actin into 50ul total volume binding buffer.Mix 5ug GST-fusio
Assay-for-the-Micrococcal-Nuclease
Method: Essentially that described by Heins et al. (1966) based upon the release of acid soluble oligonucleotides following nuclease digestion of DNA.
Glucosamine-Rapid-Assay
Glucosamine Rapid AssayMRTHOD:Place sample (containing 0.5 - 10 µg GlcN) in a Pyrex screw capped tube.Add HCl to a final concentration of 2N and a fin
LOWRY-PROTEIN-ASSAY
The Lowry procedure is one of the most venerable and widely-used protein assays, being first described in 1951 [Lowry et al., J. Biol. Chem. 193: 265-
Bradford-protein-assay
Bradford protein assayConsiderations for useThe Bradford assay is very fast and uses about the same amount of protein as the Lowry assay. It is fairly
Tube-formation-assay
DescriptionThis is a fast and easy assay to test the angiogenic/anti-angiogenic properties of molecules. As compared to other angiogenesis assays, suc
Noble-Agar-Assay
DescriptionCancer cells do not show anchorage and contact inhibition of growth. To assess the anchorage and contact independent growth of cells, noble
BIURET-PROTEIN-ASSAY
BIURET PROTEIN ASSAYMATERIALSBiuret ReagentBovine serum albumin (BSA)Spectrophotometer and tubesPROCEDUREPrepare standard dilutions of BSA containing
DNA-methyltransferase-Assay
Methylated CpG island Amplification Protocol written by Minoru Toyota2. Materials2.1. MCARestriction enzymes SmaI, XmaIT4 DNA ligaseTaq DNA polymerase
Migration-Assay-Protocol
Materials to be prepared beforehand:1) FBS free medium2) 10% FBS medium3) Cell migration filter insert ( Transwell®, 12mm Diameter, 12 μm Pore Size.)P
Adhesion-Assay-Protocol
Materials to be prepared beforehand:1) Washing Buffer--0.1% BSA in medium (DMEM or RPMI)2) Blocking Buffer--0.5% BSA in medium (DMEM or RPMI)3) Lamini
Assay-of-Phospholipase-A-Activity
Phospholipases of the A type constitute a large family of esterases that catalyze the hydrolysis of the fatty acid ester bonds in phospholipids an
Pheromone-Halo-Assay
-Use sterile technique and sterile solutions throughout this method.-1. Grow a starter culture at 30 C with shaking (250 rpm) until it reaches saturat
HISTONE-KINASE-ASSAY
PROTOCOLTo 1.5 mL eppendorf tubes add:200 µg of protein extract (see Western blot protocol for protein sample preps)q.s. to 300 µL with RIPA (with pro
Protein-Assay-(Spectrophotometer)
Protein Assay (Spectrophotometer)Use BSA (bovine serum albumin) 1mg/ml stock solution (1ml Eppendorf tubes) for standard curve.Place 0, 2, 5, 10, 15,
Cell-Viability-Assay
Dye exclusiona cell suspension is mixed with trypan blue and examined by low-power microscopyMaterialscellsPBSM3hemocytometer0.4 % trypan blue in PBSm
cell-proliferation-assay
cell proliferation assaybefore start:thaw cells from liquid nitrogen, grow in 75cc flask (T75) in Fischer's medium MM (maintenance medium) until c
ELISA-Inhibition-Assay
ELISA Inhibition AssaySensitize a 96-well microtiter plate with purified antigen.Prepare a solution of the purified antigen of interest in phosphate b
Leaf-GUS-Assay
实验概要a protocol for Leaf GUS Assay This protocol is for small samples (usually single leaf from 21DAI plants), scale up for larger samplesAs there are