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Ch 3 Lipids
Ch 3 Lipids

FischerSpr10
FischerSpr10

Determination of the Binding Site-Size of the Protein
Determination of the Binding Site-Size of the Protein

Bioinstrumentation - E
Bioinstrumentation - E

... (1) Ammeter (2) Potentiometer (3) Potentiometric recorder (4) All 16) Flame photometry is similar to ________ (1) Colorimetry (2) Spectrophotometry (3)Turbidometry (4) Nephlometry 17) The basic components used for observing emission from flames are ______ (1) Flame (2) Filter (3) Photomultiplier (4) ...
Week 11 - UW Canvas
Week 11 - UW Canvas

Nucleic Acids - Somma Science
Nucleic Acids - Somma Science

un06yhpo3rx0o1t6
un06yhpo3rx0o1t6

Teacher Guide
Teacher Guide

03 Nucleic Acids
03 Nucleic Acids

UltraClean 15 DNA Purification Kit
UltraClean 15 DNA Purification Kit

Demo notes update - UK Association for Science and Discovery
Demo notes update - UK Association for Science and Discovery

DNA - Our eclass community
DNA - Our eclass community

... DNA profiling uses the "repeat" sequences of non-coding DNA that are found between the genes that code for proteins. These sequences can vary a great deal between individuals (polymorphic). They are called short tandem repeats (STRs). The number of repeats is inherited. Therefore, unrelated individu ...
Effectivity of Betel Leaf (Piper betleL.) Gel Extract in Shortening
Effectivity of Betel Leaf (Piper betleL.) Gel Extract in Shortening

... determine the effectiveness of the betel leaf ethanol extract gel shortened bleeding time after the revocation of deciduous teeth. This research was conducted at the Department of Dental Nursing Clinic, Health Polytechnic Denpasar.This study is pure experimental research design with Completely Rando ...
Ch. 13 Genetic Engineering
Ch. 13 Genetic Engineering

...  The pattern of bands in a gel electrophoresis is known as a DNA fingerprint or a ‘genetic fingerprint’ or ‘genetic profile’  If a DNA fingerprint found in a sample of blood or other tissue at the scene of a crime matches the genetic fingerprint of a suspect, this can be used as evidence  A DNA s ...
A1987G060500001
A1987G060500001

5.36 Biochemistry Laboratory
5.36 Biochemistry Laboratory

Week 3. Gel electrophoresis and Bioinformatics
Week 3. Gel electrophoresis and Bioinformatics

... the cDNA sequences that encode these proteins. Once the protein sequences of AS1 and AS2 have been retrieved from the databases, the instructor will demonstrate how to submit these sequences to a software program that will make a three-dimensional (3-D) model of the AS1 and AS2 proteins. Before you ...
RFLP Lab Report
RFLP Lab Report

... by restriction enzymes, “sticky” or “blunt” ends are formed. Sticky ends occur when singlestranded regions of the ends are complementary, and blunt ends occur when cut are opposite each other. The size of DNA fragments generated depends on the distance between recognition sites. Though RFLP analysis ...
DNA Ladder - Swift Analytical
DNA Ladder - Swift Analytical

Applied molecular technique
Applied molecular technique

... piece of the tail. Human DNA may be analyzed using small blood samples or a few cells scraped from the inside of the cheek. The decrease in the amount of DNA required for analysis has allowed scientists to streamline the process so that DNA can be isolated in a few hours instead of a few days. Extra ...
CSU Agricultural Research Initiative
CSU Agricultural Research Initiative

Slide 1
Slide 1

Template-Directed Synthesis of Structurally Defined Branched
Template-Directed Synthesis of Structurally Defined Branched

HIS-Select Nickel Affinity Gel (P6611) - Technical - Sigma
HIS-Select Nickel Affinity Gel (P6611) - Technical - Sigma

Basic Steps of the DNA process
Basic Steps of the DNA process

... Three stages to PCR  1. Denaturation – this occurs with an increase of temperature where the weak hydrogen bonds  are broken and the double strand DNA separates into two single strands. Temperature may vary  according to enzyme and desired result (usually above 90 degrees)  2. Annealing ‐ Here the p ...
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Gel electrophoresis



Gel electrophoresis is a method for separation and analysis of macromolecules (DNA, RNA and proteins) and their fragments, based on their size and charge. It is used in clinical chemistry to separate proteins by charge and/or size (IEF agarose, essentially size independent) and in biochemistry and molecular biology to separate a mixed population of DNA and RNA fragments by length, to estimate the size of DNA and RNA fragments or to separate proteins by charge.Nucleic acid molecules are separated by applying an electric field to move the negatively charged molecules through a matrix of agarose or other substances. Shorter molecules move faster and migrate farther than longer ones because shorter molecules migrate more easily through the pores of the gel. This phenomenon is called sieving.Proteins are separated by charge in agarose because the pores of the gel are too large to sieve proteins. Gel electrophoresis can also be used for separation of nanoparticles.Gel electrophoresis uses a gel as an anticonvective medium and/or sieving medium during electrophoresis, the movement of a charged particle in an electrical field. Gels suppress the thermal convection caused by application of the electric field, and can also act as a sieving medium, retarding the passage of molecules; gels can also simply serve to maintain the finished separation, so that a post electrophoresis stain can be applied. DNA Gel electrophoresis is usually performed for analytical purposes, often after amplification of DNA via PCR, but may be used as a preparative technique prior to use of other methods such as mass spectrometry, RFLP, PCR, cloning, DNA sequencing, or Southern blotting for further characterization.
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