PreparationofSegmentedandPolarityMarkedMicrotubules
Segmented and polarity-marked microtubules are very useful for many different types of in vitro assays. Segmented microtubules are microtubules with a bright seed and dim elongated segments on both ends. Polarity marked microtubules are microtubules with a bright seed and a dim elongated segment only on one end -- the plus end. Selective elongation of one end is achieved by inclusion of NEM-treated tubulin,......閱讀全文
Preparation-of-Segmented-and-Polarity-Marked-Microtubules
Segmented and polarity-marked microtubules are very useful for many different types of?in vitro?assays. Segmented microtubules are microtubules with
Preparation-of-Segmented-and-Polarity-Marked-Microtubules
Preparation of Segmented and Polarity Marked Microtubules?Segmented and polarity-marked microtubules are very useful for many different types of?in vi
細胞組分和細胞器——細胞骨架
Fixation and Immunofluorescence of the Cytoskeleton?(Mitchison Lab)??Recycling Tubulin?(Mitchison Lab)??Labeling Tubulin and Quantifying Labeling Stoi
Flow-Cell-Assays-with-Microtubules:-Motility/Dynamics-in-Fluorescence
Flow cell assays are very useful for studying microtubule motility, microtubule dynamics, kinetochore-microtubule interactions and action of severing
Viscosity--Polymeriztion-of-Microtubules
LEVEL II Materials Tubulin (Brain extract from?Exercise 9.4) GTP ATP Viscometer Waterbath or incubator at 37° C Procedure
TEM-Visualization-of-Microtubules
LEVEL II Materials Coated grid for TEM 0.1 M ammonium acetate 5% ethanol saturated uranyl acetate Transmission electron microscope
Isolation-of-Microtubules-(Bovine-Brain)
LEVEL II Materials Freshly removed bovine brain?2 Wire sieve (tea strainer) Microtubule buffer (MT buffer) 0.1 M MES (2-(N-Morphi
細胞組分和細胞器——細胞器分離
Labeling Microtubules?(Molecular Dynamics Inc.??)Microtubules are involved in many aspects of cell motion including propulsion, mitosis, growth, and o
Fixation-and-Embedding-of-Microtubules-for-Electron-Microscopy
(This procedure can also be used for virtually any material that must be pelleted prior to fixation and thin sectioning) Primary fix: 2% glutaralde
Negative-Stain-Electron-Microscopy-of-Microtubules
Negative staining is a rapid, qualitative method for analyzing microtubule structure at the EM level. Because negative staining involves deposition of
Preparation-of-tubulin
Although many protocols for tubulin preparation are available, the procedure described below is the simplest and highest yielding preparation I have
SMEAR-PREPARATION
The preparation of a smear is required for many laboratory procedures, including the Gram-stain. The purpose of making a smear is to fix the bacteria
Platelet-Preparation
OUTLINEIn order to avoid platelet activation all manipulations must be performed as quickly and as acurate as possible.Work on ice if possible!?This p
Template-Preparation
Template PreparationThe quality of sequencing results is directlyrelated to the quality of the template.?ABI recommends a minialkaline-lysis/PEG preci
Liposome-Preparation
Liposome PreparationOBJECTIVE:Method for incorporating proteins into liposomes for liposome swelling assay or as an alternative antigen presentation m
CAM-preparation
8 eggs per day, day 7- day 13?cut CAM, wash in precooled PBS,in 10 ml WASH 1 (PBS, 5 mM EDTA, COMPLETE) on icecut in pieces in petri dish on icecentri
Ultraviolet-irradiation-impairs-epiboly-via-microtubules-in-Zebrafish
Introduction Zebrafish have transparentembryos that develop outside the mother. They develop rapidly, so that at 24 hours after fertilization, the em
MARK2基因編碼功能及結構描述
該基因編碼絲氨酸/蘇氨酸蛋白激酶Par-1家族的一個成員該蛋白是上皮細胞和神經元細胞極性的重要調節因子,通過磷酸化和失活多種微管結合蛋白來調控微管的穩定性。蛋白質定位于細胞膜已發現該基因編碼不同亞型的多個轉錄變體。[由RefSeq提供,2009年7月]This gene encodes a memb
MAPK2基因突變與藥物因子介紹
該基因編碼絲氨酸/蘇氨酸蛋白激酶Par-1家族的一個成員該蛋白是上皮細胞和神經元細胞極性的重要調節因子,通過磷酸化和失活多種微管結合蛋白來調控微管的穩定性。蛋白質定位于細胞膜已發現該基因編碼不同亞型的多個轉錄變體。[由RefSeq提供,2009年7月]This gene encodes a memb
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
Metaphase-chromosome-preparation
Materials:? RPMI 1640 medium? fetal calf serum (FCS), 20%? Colcemid (e.g. Boehringer Mannheim cell biology reagents, Best.-Nr. 295892)? cell cuture f
PREPARATION-OF-MICROINJECTION-PIPETTES
INJECTION AND HOLDING PIPETTES The glass capillary tubing used should be thin walled, borosilicate glass without a fibre. e.g. Clark Electromedical
Preparation-of-Polyacrylamide-Gels
1. Prepare 20X TBE as: 216 g Tris Base 110 g Boric Acid 80 mL 500 mM EDTA, pH 8.0 700 mL ddH2O Mix. Bring volume to 1 L. Autoclave. 2. Prepare Acry
Preparation-of-Agar-plates
Prepare media and add 1.5 agar before autoclaving it (15g per liter).? After autoclavation, cool the media in a 55 degree waterbath. Do not allow? th
DGK-Membrane-Preparation
Reagents: Bacterial strain E.?coli N4830/pJW10 LB amp media 50 μg/ml ampicillin High salt buffer for 1 L 50 mM KH2PO4 6.8 g 150 mM KCl 11.18 g 50
Preparation-of-Mouse-Neutrophils
實驗概要Preparation of Mouse Neutrophils實驗步驟Mice:8-16 weeks old malePrewarm buffer to room temperatureBuffer A : Ca2 ?/Mg2 ‐free Hank’s buffered saline so
Rat-Liver-Preparation
實驗概要The procedure presented below describes a method for preparing rat liver.主要試劑1.????? Aluminum Foil2.????? Liquid Nitrogen3.????? Dry Ice4.????? Ph
Preparation-of-Phage-Lysates
Preparation of Phage LysatesInoculate 5 ml of lambda-broth in a glass culture tube with a single colony of an appropriate host strain of?E. coli. Incu
Preparation-of-Mouse-Neutrophils
實驗步驟Mice:8-16 weeks old malePrewarm buffer to room temperatureBuffer A : Ca2 ?/Mg2 ‐free Hank’s buffered saline solution [HBSS; Invitrogen, Grand Isla
PREPARATION-OF-SEQUENCING-GELS
MATERIALS:2-glass plates1 sharks -tooth comb and spacersWhatman 3 mm paper30 or 40% acrylamide-bis (19:1)10X TBEurea10% ammonium persulfateTEMED60 cc.