SUMMARY The steady state kinetics of initiation of T7 DNA transcrip

... Nucleic Acids Research schema it is possible that one of the routes if favored under normal conditions, but all of them are principally possible. This would be called a kinetically ordered mechanism. One could also think about "mixed-type" mechanisms, in which substrates bind randomly, while produc ...

- Catalyst

... PM a. Pore-forming toxins ...

MagExtractor -Plasmid

... (13) Place the tube in the magnetic stand and collect the beads with the magnet. (14) After magnetic capture, carefully remove the supernatant. (15) Repeat (12) - (14) (16) optional Evaporate EtOH by heating the opened microtube to 78°C for ≤ 15 minutes. ...

Proposal Submission Form

... rDNA: involving eukaryotic viruses (not more than 2/3 genome) in cell culture, used with whole plants (low risk work) and associated small animals, arthropods, or generation of transgenic rodents (BSL1), any work not covered in the other categories (most non-pathogenic rDNA work) rDNA: not in organi ...

DNA copy number analysis by MAPH: molecular diagnostic

... locus at a chromosome end, is shown as a peak. The first sam- BRCA1 or subtelomeric DNA analysis, however, the exon or ple is a heterozygous deletion of 17q (17q-) and the second is chromosome end that varies, if any, is not known. This can be an unbalanced translocation between chromosomes 16 and 3 ...

PCR primers for the amplification of the nuclear small subunit

... central capsular wall. The central capsule contains major cytoplasmic organelles: nucleus, mitochondria, and other membranous organelles, exclusive of digestive vacuoles (Anderson, 1983). Symbiotic algae are generally found in the ectocytoplasm. ...

One Shot PIR1 and PIR2 - Thermo Fisher Scientific

... contained in the One Shot® Kit. This can be accomplished by using the supercoiled pUC19 plasmid supplied with the kit as described below. • Prepare LB agar plates containing 100 µg/ml ampicillin • Transform 1 µl (10 pg) into 50 µl of competent cells according to the transformation protocol on the pr ...

BIO 101 Lab OBJECTIVES

... 2. Know how positive and negative controls are used. 3. Know the subunits that make up these 4 groups: carbohydrates (monosaccharides, disaccharides and polysaccharides), proteins, lipids and nucleic acids. 4. Know what the following reagents are used to test for and what a positive result would loo ...

Chapter 18

... Chapter 18 - Genetics of Viruses and Bacteria NEW AIM: Viruses: Packaged Genes… Influenza looks different…it has an envelope. What’s up with that? ...

Horizontal Gene Transfer between Bacteria

... ‘Transfer’ refers to translocation of genetic material into a cell, followed by stable integration into the recipient genome, including autonomously-replicating components of the genome (e.g. a plasmid, accessory chromosome or organelle chromosome). The transferred gene can be perpetuated in the off ...

Review Article The biosafety of molecular farming in plants

... the costs associated with molecular farming in plants are due to postharvest processing and compliance with regulatory procedures. Product safety compared to traditional expression systems In terms of product safety, animal-based expression systems run the risk of harbouring pathogens and undesirabl ...

View

... The positioning patterns of γ-H2AX in Jurkat cells indicate that sub-telomeric and actively transcribed regions are sensitive to endogenous DNA damage. Sub-telomeres are known to be prone to replication-mediated DSBs, particularly due to oncogenic replication stress (10,11). DNA hyperreplication in ...

Greedy Algorithms

... • The mouse genome can be cut into ~300 (not necessarily equal) pieces and joined pasted together in a different order (“rearranged”) to obtain the gene order of the human genome • Synteny blocks • Synteny blocks from different chromosomes in mouse are together on the same chromosome in human ...

Rapid generation of nested chromosomal

... Making nested deletions directly in mice, however, generally has been limited to regions containing visible markers (2, 10). In addition, large numbers of mice need to be screened to recover multiple deletions at the same locus (11). The ability to induce deletions in embryonic stem (ES) cells and t ...

exercises - Evolutionary Genomics Group

... The way of comparing the 16 sRNA sequences is to do a multiple sequence alignment. In this course we use clustal to align the sequences and find the distance/differences between them. The greater the distance between two sequences the greater the difference between the organisms from which the seque ...

Generation and analysis of mutated clonal scFv Jiya George

... Human immuno deficiency virus (HIV) incorporates host cellular protein, beta-2-microglobulin (β2m), into its surface envelope during budding. β2m is a cellular protein that belongs to the major histocompatibility complex (MHC) Class I molecules. Studies have shown anti-β2m monoclonal antibodies (mAb ...

KARNATAKA COMMON ENTRANCE TEST – MAY, 2016 BIOLOGY

... Disclaimer: These solutions are provided by the academic team of BASE. These solutions may be different from those to be provided by the Karnataka Examinations Authority (KEA) due to difference in assumptions taken in support of the solutions. In such cases solution provided by KEA will be deemed as ...

Types of variation in DNA-A among isolates of East African cassava

... genes apparently can have a different evolutionary origin from complementary-sense genes, and ori seems to be a recombination hot spot, occurs among begomoviruses infecting cotton and okra in Pakistan (Zhou et al., 1998). If the same is true for EACMV, the extent of the sequence dissimilarity betwee ...

srep09383-s1

... confirmed by confirmed by restriction analysis with BglII after stable propagation through E. coli (Figure S5). Genetic manipulation of the ami genes. Genetic manipulations were carried out using λ-Red recombination-mediated PCR targeting 4. The amiA and amiB genes on pCAPB2-ami were individually re ...

Encyclopedia of Nanotechnology

... accessible by conventional techniques, such as scanning-force-microscopy-based techniques (in aqueous/ liquid environment, the natural “habitat” for many both in vitro and in vivo biological systems), OT has become a major investigating tool in biology (for recent reviews on instrumentation in optic ...

Collaborative coupling between polymerase and helicase for

spectroscopic studies of mosquito iridescent virus, its capsid

... size distribution and an accessible core below 80 nm in diameter [1]. Optical spectroscopy is one of the efficient and informative methods of studying viruses. It provides well reproducible results and is a powerful supplement to conventional biological methods of studying the living organisms. Thus ...

infection

... Dr. Jenna Collins rounded the corner of the hospital hallway and entered her next patient’s room. There she saw Kayla Starnes lying in the hospital bed in front of her with her mother standing nearby. Picking up Kayla’s chart, Dr. Collins introduced herself to Kayla. “Hi, I’m Dr. Collins. I hear you ...

File

... 1. Garrod hypothesized that "inborn errors of metabolism" such as alkaptonuria occur because a. metabolic enzymes require vitamin cofactors, and affected individuals have significant nutritional deficiencies. b. enzymes are made of DNA, and affected individuals lack DNA polymerase. c. many metabolic ...

Restriction Enzymes Brochure

... restriction enzymes: buffer compatibility and star activity. HF restriction enzymes have 100% activity in CutSmart™ Buffer; singlebuffer simplicity means more straightforward and streamlined sample processing. HF enzymes also exhibit dramatically reduced star activity. Engineered with performance in ...

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Cre-Lox recombination

In the field of genetics, Cre-Lox recombination is known as a site-specific recombinase technology, and is widely used to carry out deletions, insertions, translocations and inversions at specific sites in the DNA of cells. It allows the DNA modification to be targeted to a specific cell type or be triggered by a specific external stimulus. It is implemented both in eukaryotic and prokaryotic systems.The system consists of a single enzyme, Cre recombinase, that recombines a pair of short target sequences called the Lox sequences. This system can be implemented without inserting any extra supporting proteins or sequences. The Cre enzyme and the original Lox site called the LoxP sequence are derived from bacteriophage P1.Placing Lox sequences appropriately allows genes to be activated, repressed, or exchanged for other genes. At a DNA level many types of manipulations can be carried out. The activity of the Cre enzyme can be controlled so that it is expressed in a particular cell type or triggered by an external stimulus like a chemical signal or a heat shock. These targeted DNA changes are useful in cell lineage tracing and when mutants are lethal if expressed globally.The Cre-Lox system is very similar in action and in usage to the FLP-FRT recombination system.

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Cre-Lox recombination