We narrowed to 809 results for: TES

Production of Virus in Insect Versus Mammalian Cells

• Published: Nov. 5, 2024, 8:32 p.m.

...to collect your viral supernatant. Baculovirus replicates inside insect cells, and its lifecycle ends in...

Viral Vectors 101: Producing Your rAAV

• Published: July 16, 2024, 1:15 p.m.

..., E., Hernandez, A., Boye, S. L., Boye, S. E., Levites, Y., … Golde, T. E. (2020). Utilizing minimally...

Antibodies 101: Flow Compensation

• Published: May 16, 2024, 1:15 p.m.

...diagonal population, this is a sign of spillover and indicates that it is necessary to apply a compensation value...

Twenty Years of Addgene Sharing: CRISPR

• Published: April 18, 2024, 1:15 p.m.

... and the longevity of tools seen in Figure 3, indicates that the usefulness of popular CRISPR tools is...

Antibodies 101: Conventional vs Spectral Flow Cytometry

• Published: Aug. 3, 2023, 1:15 p.m.

...AntibodiesAntibodies 101: Buffers, Storage, and Conjugates Resources on Addgene.org Addgene's Antibody GuideAddgene's...

Academic vs. Industry Postdocs

• Published: Nov. 13, 2018, 1:22 p.m.

... companies, such as Novartis, have specific web sites for postdoc listings, so the method of posting varies...

AAV Vector Quality Control: Going the Extra Mile with NGS

• Published: Sept. 12, 2017, 1:44 p.m.

...Vector Characterization Methods for Quality Control Testing of Recombinant Adeno-Associated Viruses. In: Methods...

Quick Guide to Working with Drosophila Part 1: Getting Started with Flies

• Published: July 13, 2017, 2:30 p.m.

... systems. Some resources will direct you to the latest information about gene function, while others offer...

Fluorescent Proteins 101: Visualizing Subcellular Structures & Organelles

• Published: June 22, 2017, 2:30 p.m.

...localization and transport between healthy and diseased states can also provide interesting insights into disease...

Plasmids 101: Protein Expression

• Published: June 7, 2018, 1:17 p.m.

...Production of recombinant proteins in plant root exudates Resources on the Addgene Blog Learn about inducible...

Anatomy of a Plasmid Page at Addgene

• Published: Feb. 4, 2016, 3:30 p.m.

...is an indication of popularity. A yellow flame indicates that a plasmid has been ordered more than 20 times...

A Guide to Starting Your Own Journal Club

• Published: Feb. 6, 2020, 3 p.m.

...scheduling conflicts. This helped us find a time that accommodates more people. The feedback could be solicited...

Transferable Skills Guide: Identifying Your Transferable Skills

• Published: Jan. 11, 2018, 3:29 p.m.

...about your communication style, your potential teammates want to be assured that you will contribute openness...

New Optimized Genome-wide CRISPRko, CRISPRi, and CRISPRa Libraries

• Published: Oct. 4, 2018, 12:44 p.m.

...effects in human genomes (Doench et al., 2016). To test the library, they conducted genome-wide negative...

Lentiviral Vector Uses and Overview

• Published: May 19, 2016, 2:30 p.m.

...transcriptional activation from the 5’ LTR) and Rev (facilitates nuclear export of transcripts). A different viral...

CRISPR Antimicrobials

• Published: May 3, 2016, 2:30 p.m.

...the world is unprepared. Each year in the United States, two million people will be infected by antibiotic...

Interview: Hodaka Fujii on enChIP, New CRISPR Tools, and More

• Published: Dec. 2, 2014, 7:23 p.m.

...early research career. I've found that research institutes in different places have very different cultures...

Your Lentiviral Plasmid FAQs Answered

• Published: April 23, 2014, 1:08 p.m.

...envelope plasmid you use as the choice of envelope dictates the tropism of the virus.  VSV-G is very common...

Twenty Years of Sharing: Addgene's Viral Vector Service

• Published: July 30, 2024, 1:15 p.m.

...protein tools that are activated, respectively, by substrates, light, or engineered ligands (Figure 2). Biosensors...

Viral Vectors 101: Preparing Pooled Libraries

• Published: July 13, 2023, 1:15 p.m.

...amplification. Transformed E. coli are allowed to grow on plates or in liquid culture to amplify the library, followed...