Metaphasechromosomepreparation
Materials: RPMI 1640 medium fetal calf serum (FCS), 20% Colcemid (e.g. Boehringer Mannheim cell biology reagents, Best.-Nr. 295892) cell cuture flask Phythemaglutinin, PHA-L (Seromed, M 5030) CO2 cell culture incubator 50 ml Nunc/Falcon tubes 15 ml Nunc/Falcon tubes KCl (0.075 M, 0.055% ?) Fixative (methanol/acetic acid 3 : 1) glass microscopy slidesAmounts ......阅读全文
Preparation-of-Plasmid-DNA-by-Alkaline-Lysis-with-SDS:-Maxipreparation
实验概要Plasmid DNA is isolated from large-scale (500 ml) bacterial cultures by treatment with alkali and SDS.主要试剂Buffers and SolutionsAlkaline lysis solu
96Well-Sample-Preparation-for-Adherent-Cells
实验概要The procedure presented below describes a facile method for studying signal transduction events with adherent cells (HeLa, MCF-7, BALB/c 3T3, et
Preparation-of-denaturing-6%polyacrylamide-gels-for-microsatellite-analysis
Preparation of denaturing 6% polyacrylamide gels for microsatellite analysis(also for SSAP, high-resolution IRAP/ISSR and other analyses)Saadiah Jamli
96Well-Sample-Preparation-for-Suspension-Cells
实验概要The procedure presented below describes a facile method for studying signal transduction events with suspension cells (Jurkat, Raji, THP-1, etc.
Isolation-of-human-multipotent-mesenchymal-stem-cells-from-second
Isolation of human multipotent mesenchymal stem cells from second‐trimester amniotic fluid Culture of MSC from amniotic fluid1. Twenty amniotic flui
组织学——组织制备
· Histological techniques (William H. Heidcamp)Very detailed guide to histological techniques, like fixation, dehydration, embedment and subs
细胞遗传学——原位引物启动技术(PRINS)
· Hiro Hirai's Primed in Situ Synthesis (Schistosoma Genome Network)The PRINS (Primed in situ) technique uses a specific primer, dNTPs wit
Optimized-Method-for-the-Preparation-of-Rodent-Testicular-Cells1
Homogeneity of cell populations is a prerequisite for the analysis of biochemical and molecular events during male gamete differentiation. Given the c
A-practical-method-for-the-preparation-of-total-DNA-from-filamentous-fungi
Most methods of DNA preparation from fungi are time-consuming due to the need to first make protoplasts, expensive for chemicals such as cesium chlori
Optimized-Method-for-the-Preparation-of-Rodent-Testicular-Cells3
Moreover, when the method was applied to the analysis of the cellular composition of immature testes, the results were also in agreement with previous
Preparation-of-cytoplasmic-extracts-for-the-application-inacellfree-system
Characteristics of this procedure:Cells are grown to 80% confluency, then harvested, washed and disrupted in KPM buffer by freezing-thawing cycles wit
Optimized-Method-for-the-Preparation-of-Rodent-Testicular-Cells2
Flow Cytometric AnalysisPrior to flow cytometric analysis, the vital dye Hoechst 33342 (Sigma-Aldrich, St. Louis, MO, USA) was added to cell suspensio
Method:-Preparation-of-Lymphoblastoid-Cell-Lines-for-Long-Term-Storage
Method: Preparation of Lymphoblastoid Cell Lines for Long Term StorageMay 30, 1990Rosalie VeilePurpose:To store cell lines in a form that will insure
Preparation-of-High-Titer-Adenovirus-in-P11-cells
adapted from Cell Biology, A Lab Manual, second edition, volume 1 -Grow up P11 cells in 15 cm plates to 70 – 80% confluence. -Infect cells with a MOI
Preparation-of-Bacterial-Proteins-for-Analysis-by-2DPAGE
The following protocol has been developed for preparing soluble bacterial proteins in a form suitable for analysis by 2D-PAGE. The procedure was princ
Method:-Reactivating-Cell-Lines-and-Cell-Growth-for-DNA-Preparation
Purpose:Cell lines are reactivated and grown to a count of 1 x 108 cells. The cells are pelleted and stored frozen at -80 degrees C prior to DNA extra
Cosmid-Cloning:-Cell-preparation,-DNA-packaging,-and-Cell-Transfection
Cosmid Cloning: Cell preparation, DNA packaging, and Cell TransfectionProtocol taken from Stratagene's Gigapack packaging extracts instruction man
STAG1基因编码的功能和结构描述
该基因是scc3家族的一员,在细胞核中表达。它编码一种多亚单位蛋白质复合物-黏着素的成分,这种复合物通过前期和前期的DNA复制,沿着染色体长度提供姐妹染色单体的黏着,然后在后期分离。This gene is a member of the SCC3 family and is expressed i
CGH-Protocols-(三)
Hybridizationreagents: labeled tumor and normal-DNA (see protocol Nick translation) salmon sperm DNA, 10 mg/ml (e.g. Promega) human Cot1 DNA, 1 mg/ml
STAG1基因突变因子与药物介绍
该基因是scc3家族的一员,在细胞核中表达。它编码一种多亚单位蛋白质复合物-黏着素的成分,这种复合物通过前期和前期的DNA复制,沿着染色体长度提供姐妹染色单体的黏着,然后在后期分离。[由RefSeq提供,2008年7月]This gene is a member of the SCC3 family
Preparation-of-cytoplasmic-extracts-forthe-application-in-acellfree-system
DescriptionCells are grown to 80% confluency, then harvested, washed and disrupted in KPM buffer by freezing-thawing cycles with liquid nitrogen essen
Protocols-for-the-preparation-of-tumour-cells-for-s.c.-injections-in-mice
For the establishment of solid tumour in nude mice, tumour cells are treated in a sterile environment under a cell culturing hood. Disposable sterile
Protocols-for-the-preparation-of-tumour-cells-for-s.c.-injections-in-mice
For the establishment of solid tumour in nude mice, tumour cells are treated in a sterile environment under a cell culturing hood. Disposable sterile
Mapping-Protein-Distributions-on-Polytene-Chromosomes-by-Immunostaining1
INTRODUCTIONThe formidable size and structure of polytene chromosomes allowmapping of chromosomal protein distributions at very high resolution.This p
蛋白质提取与制备(Protein-Extraction-and-Preparation)2
三、蛋白质提取与制备具体操作方法1、原料的选择早年为了研究的方便,尽量寻找含某种蛋白质丰富的器官从中提取蛋白质。但至目前经常遇到的多是含量低的器官或组织且量也很小,如下丘脑、松果体、细胞膜或内膜等原材料,因而对提取要求更复杂一些。原料的选择主要依据实验目的定。从工业生产角度考虑,注意选含量高、来源丰
Preparation-of-Genomic-DNA-from-Bacteria-using-Phase-Lock-GelTM
Preparation of Genomic DNA from Bacteria- using Phase Lock GelTM (Modified from Experimental Techniques in Bacterial Genetics, Jones and Bartlet, 1990
蛋白质提取与制备(Protein-Extraction-and-Preparation)4
蛋白质提取液中,除包含所需要的蛋白质(或酶)外,还含有其它蛋白质、多糖、脂类、核酸及肽类等杂质。除去的方法有:1)核酸沉淀法该法可用核酸沉淀剂和氯化锰、硫酸鱼精蛋白或链霉素等。必要时也可用脱氧核糖核酸酶除去核酸。即在粗匀浆中加入少量DNase,于4℃保温30~60min,可使DNA 降解为足够小的碎
反向微柱的准备Preparation-of-ReversedPhase-Microcolumns
INTRODUCTIONOne versatile strategy for sample cleanup prior to MALDI-MS analysis uses microscale columns designed for direct sample elution onto the M
蛋白质提取与制备(Protein-Extraction-and-Preparation)6
PH 值:与沉淀蛋白质或酶原理相同,结晶的溶液PH 值一般选择在被结晶的蛋白质或酶的等电点附近,以利于晶体的析出。温度:除少数情况外,通常选择低温条件进行。低温条件对蛋白质和酶不仅溶解度低且不易变性。在中性盐溶液中结晶时,温度可在0℃至室温范围内选择,在有机溶剂中结晶一般要求温度较低。晶种:不易结晶
蛋白质提取与制备(Protein-Extraction-and-Preparation)5
确定沉淀蛋白质所需硫酸铵浓度的方法将少量样品冷却到0~5℃,然后搅拌加入固体硫酸铵粉末,见蛋白质产生沉淀时,离心除去沉淀,分析上清液确定所要蛋白质的浓度,如它仍在溶液中则弃去沉淀,再加更多的硫酸铵于上清液中,直到产生蛋白质沉淀时止。以所要提取的蛋白质在溶液中的浓度对硫酸铵浓度作图,得沉淀曲线,找出蛋