Author: admin

Overview DNase I is an endonuclease that selectively cleaves phosphodiester bonds of both single- and double-stranded DNA without cleaving RNA….

DNA-free RNA preparations are absolutely required for applications like gene expression analysis using PCR-based methods (e.g., real-time PCR). No RNA…

Overview: In molecular biology laboratories, IPTG is commonly used to induce the expression of recombinant proteins in E. coli and…

Overview   Organism Mouse (Mus musculus) Source/Tissue Melanoma Morphology Epithelial-like Cell type   Growth mode Adherent, monolayer Doubling time ≈…

OVERVIEW   Organism Human (Homo sapiens), 1 year old, female Source/Tissue Muscle, rhabdomyosarcom Morphology Epithelial-like Cell type   Growth mode…

Overview: Phenol is a colorless crystalline solid. Phenol gradually turns pink to brownish color due to oxidation upon exposure to…

A 100 ml of 4% (w/v) paraformaldehyde can be prepared by dissolving 4g of paraformaldehyde in PBS to a final volume of 100 ml.

♦ After the gel electrophoresis has been completed, the next step is to analyze agarose gel for DNA fragments. Unfortunately,…

There are many nucleic acid staining dyes that can be used to visualize DNA embedded in the agarose gel. These…

Overview Preparation of metaphase chromosome spread is an important technique in cytogenetics. Metaphase chromosome spread is used for karyotyping including…

The serum is commercially supplied in different sizes with 500 ml being the most common size. Since repeated freezing and…

Ready to use L-glutamine solution (200 mM, sterile-filtered, 100 x concentration) is commercially supplied in different sizes with 100 ml…

Laminar flow hood (Class II) provides a sterile environment for handling cell culture. To make the laminar flow hood ready…

Overview Heat inactivation of serum refers to the process which involves treatment of serum at a higher temperature to inactivate…

Complete replacement of culture medium from suspension culture involves cell harvesting by centrifugation and resuspension of the cell pellet in fresh growth medium. This method is ideally the best way to feed suspension culture and is often used when a. you observe dead or sick cells/suspended particles in culture; b. medium color (phenol red-containing medium) has turned yellow very quickly; c. you can not afford cell loss. Complete replacement of culture medium is ideally the best way to feed suspension culture. Since this procedure takes time and involves an additional centrifugation step to harvest cells, often researchers partially replace the medium that takes just a few minutes. However, partial medium replacement is associated with the loss of cells from the culture.