TUNELPROCEDUREINBOVINEEMBRYOS
Materials8% (w/v) paraformaldehyde stock solution: Dissolve 8 g of powdered paraformaldehyde in 100 ml water. Heat and stir (55-60 C – do not go higher). Add a few drops of 2 N sodium hydroxide until the solution clears. Make fresh each day. Alternatively, 8% paraformaldehyde can be purchased from Electron Microscopy Sciences as a custom formulation in 4 ml aliquots (cat. no. 157......阅读全文
TUNEL-PROCEDURE-IN-BOVINE-EMBRYOS
Materials8% (w/v) paraformaldehyde stock solution: Dissolve 8 g of powdered paraformaldehyde in 100 ml water. Heat and stir (55-60 C – do not go high
TUNEL-PROCEDURE-IN-BOVINE-EMBRYOS
Materials8% (w/v) paraformaldehyde stock solution: Dissolve 8 g of powdered paraformaldehyde in 100 ml water. Heat and stir (55-60 C – do not go high
Tunel-Procedure-in-Bovine-Embryos-牛胚胎TUNEL检测凋亡
Materials8% (w/v) paraformaldehyde stock solution: Dissolve 8 g of powdered paraformaldehyde in 100 ml water. Heat and stir (55-60 C – do not go highe
发育生物学
In Vitro Production of Bovine Embryos (P.J. Hansen Lab, Dept. of Animal Sciences, University of Florida)This protocol describe procedures for in vitro
Whole-mount-TUNEL-analysis-of-Xenopus-embryos
Fixation and pretreatmentDejelly albino embryos carefully in 2% Cystein (pH 7.8).Remove the vitellin membrane with two pairs of tweezers (or c
Isolation-of-Microtubules-(Bovine-Brain)
LEVEL IIMaterialsFreshly removed bovine brain 2Wire sieve (tea strainer)Microtubule buffer (MT buffer)0.1 M MES (2-(N-Morphilino)ethanesulfonic acid)1
多功能胚胎激光破膜仪(二)
A new approach to cyropreservation of large equine embryos by vitrification after blastocoel micromanipulation.J. Scherzer, R. A. Fayrer-Hosken, L. Ra
Fixation-of-Embryos
MEMFA Fix10xMEMFA Salts1 part 10x MEMFA salts1 M MOPS1 part 37% formaldehyde20mM EGTA8 parts water10mM MgSO410x salts can be autoclaved and stored. Tu
多功能胚胎激光破膜仪(一)
Laser-assisted derivation of human embryonic stem cell lines from IVF embryos after preimplantation genetic diagnosis.T. Turetsky, E. Aizenman, Y. G
In-Vivo-Luciferin-Imaging-Procedure
Mice are injected by an intraperitoneal route with a Luciferin solution (15 mg/mL or 30 mg/kg, in PBS, dose of 150 mg/kg) that is allowed to distribut
DNA-EXTRACTION-PROCEDURE--GENERAL
Grow cells overnight in 500 ml broth medium.Pellet cells by centrifugation, and resuspend in 5 ml 50 mM Tris (pH 8.0), 50 mM EDTA.Freeze cell suspensi
Gramstaining-Procedure
Gram-staining is a four part procedure which uses certain dyes to make a bacterial cell stand out against against its background. The specimen should
Isolation-of-mouse-embryos
1. Sacrifice impregnated mouse.2. Dissect out the uterus of the mouse. Pulling up on the uterus with one set of forceps,use another to tear the mesome
Isolation-of-Zebrafish-embryos
Zebrafish will mate and deposit fertilized eggs on the bottom of the tank at 'dawn'. They can be accustomed to lay at any convenient time by k
Wholemount-staining-of-embryos
Fix embryos in formalin or MEMFA for one hour at room temperature with mixing. Rinse with TBS, replace with methanol, store at -20oC.Rehydrate by slow
细胞凋亡(TUNEL,TUNEL染色)检测技术
细胞凋亡是指为维持内环境稳定, 生物体内细胞在特定的内源或外源信号诱导下,其死亡途径被激活,并在有关基因的调控下发生的程序性死亡过程。细胞凋亡是程序性死亡过程的一种主要形式,它涉及染色质凝聚和外周化、细胞质减少、核片段化、细胞质致密化、与周围细胞联系中断、内质网与细胞膜融合,最终细胞片段化形成许多
Culture-of-BEND-Cells-(Bovine-Endometrial-Cells)
Culture of BEND Cells (Bovine Endometrial Cells)Charles E. Krininger, III and Peter J. Hansen Dept. of Animal Sciences, University of FloridaThis prot
TUNEL-labeling
In Situ Cell Death (Apoptosis) Detection by TUNEL labelingby Boehringer Mannheim (Catalog No. 1684809), modified by Josiah N. Wilcox andJosé C. Rodrig
TUNEL-方法
Terminal deoxynucleotidyl Transferase-mediated dUTP nick end labeling (TUNEL) is an in situ method for detecting the 3'-OH ends of DNA exposed dur
TUNEL-assay
PROTOCOL:•Deparaffinize and rehydrate slides:3 x 3´ Xylene3 x 2´ 100% ethanol1 x 2´ 95%, 80%, 70% ethanol (each)1 x 5´ 1x PBS•Microwave antigen retrie
TUNEL分析实验——组织切片的-TUNEL-染色
实验材料组织试剂、试剂盒甲醛NaOHPBS二甲苯乙醇蛋白酶 KTris-HCl 溶液仪器、耗材Parafilm 膜实验步骤1. 取下组织,立即用新制备的 4% 甲醛固定,室温过夜。用多聚甲醛制备 4% 的甲醛溶液,在 100 ml 水中加 8 g 多聚甲醛,在通风橱中加热至 50~60℃,加几滴 1
Protocol-to-Count-Cell-Number-of-Preimplantation-Embryos
Protocol to Count Cell Number of Preimplantation Embryos using Nuclear Staining with Hoechst 33342 or DAPI Introduction The following is a simple pro
James-Hardwick-CNBr-Cleavage-Procedure
1. Immunoprecipitate the protein and run it on a preparative gel. CNBr cleavage must be done with protein transferred to a nitrocellulose filter. Neit
An-Integrative-Procedure-for-Apoptosis-Identification-and-Measurement
IntroductionApoptosis is a normal physiological phenomenon put forward by Kerr [1]. It plays an important role in embryonic development, maintenance o
Obtaining-Embryos:-hCG-Injection
Ovulation is induced in X. tropicalis by injection of human chorionic gonadotropin (hCG). X. tropicalis requires a much smaller dose than does X. laev
Sectioning-stained-embryos.
The protocols for plastic and wax sections as used by the Vize lab. These protocols work, but they have not been optimized. If anyone has better proto
In-vitroculture-of-early-chick-embryos
1. Use sterile technique. Prewarm Howard's Ringers in petri dish andagar/albumin culture dish to 37ºC.2. Crack 2-day egg into large sterile petri
TUNEL分析实验——贴壁细胞的-TUNEL-染色
实验材料细胞试剂、试剂盒PBSTdT 反应混合液仪器、耗材Parafilm 膜实验步骤1. 用无菌镊子将一无菌盖玻片放入 35 mm 培养皿中。2. 将大约 1X104 细胞接种于无菌盖玻片上,培养 24~48 小时。凋亡诱导时,细胞铺满不超过 80%。如细胞贴壁不太好,可以用纤连蛋白、聚赖氨酸或血
器官培养
In vitro organ cultures (Nagy Lab)kidneylungslimb In Vitro Differentiation of ES Cells into: (Nagy Lab)Cardiac MuscleNeuronal LineagesCystic Embryoid
Development-of-the-Heart-Morphogenetic-Field-in-the-Axolotl-Embryo
IntroductionThere are two modes of development common to most species in the animal kingdom.Virtually all embryos undergo both mosaic and regulative d