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    In this experiment we used gel electrophoresis to separate goat‚ sheep‚ cow‚ horse‚ chicken serum along with cow transferrin and cow gamma globulins. In this lab we successfully prepared the gel electrophoresis bed and successfully separated the proteins. The western blot along with the nitrocellulose blot was successful but produced no visible results. Introduction: Amino acids are basic units and building blocks of proteins. They consist of an amine group‚ a carboxylic group and side chain.

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    The two techniques that were used to create a DNA profile in this experiment were PCR and gel electrophoresis. The PCR is used to amplify the several DNA samples and gel electrophoresis is performed to separate the DNA fragments according to their size. [6] In the first part of the experiment‚ PCR amplification of the DNA templates was performed and the products obtained were used to perform gel electrophoresis. The process of PCR allows for the amplification of the DNA samples and the components needed

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    Agarose gel electrophoresis is a technique used in the laboratory to separate macromolecules such as nucleic acids and proteins. Electrophoresis can take a mixture of macromolecules of different molecular weights‚ shapes‚ and various electrical charges to determine all the various compounds in the mixture and allowing for further purification that can aid in details of individual elements of the mixture being studied. Agarose gel electrophoresis is a very important technique used in the field of

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    Gel Electrophoresis is used to separate the haemoglobin component of blood. Because each type of haemoglobin (HbA‚ HbS‚ Hbc and more) have different electrical charges‚ they will separate after undergoing gel electrophoresis. Firstly‚ a blood sample from the patient is taken and is applied to a cellulose acetate membrane strip that has been soaked in a buffer solution along with saponin. The red blood cells are lysed by the saponin while being soaked‚ therefore they release their haemoglobin. A

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    agarose gel electrophoresis in an emulation of DNA fingerprinting. The task‚ which was successfully carried out was to determine whether DNA from suspects A‚ B or C matches the sample of blood found at the murder scene (X). The process of PCR acts in the same way as DNA replication but is restricted to specific DNA samples of interest. By amplifying the necessary DNA sequence‚ this procedure is able to produce a usable DNA sample for agarose gel electrophoresis. Agarose gel electrophoresis is a method

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    Gel Electrophoresis Lab

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    Function 16 October 2014 Gel Filtration and Electrophoresis Objective The essential goal of the experiment was to separate proteins in a solution based on size in different fractions. The relative protein content for each one fraction was found through the utilization of an amido black-based protein assay. Later in the trial polyacrylamide gel electrophoresis was utilized to separate BSA from hemoglobin. Methods I. Gel Filtration and Protein Assay: 1. A slurry of Bio-Gel P-100 beads in water was

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    Gel Electrophoresis Lab

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    Gel Electrophoresis Lab SBI4U1 May 13th‚ 2013 Gel Electrophoresis Lab Purpose: The purpose of this lab is to learn how restriction enzymes cut DNA molecules at specific sequences‚ thus producing DNA fragments of various lengths. Students learn how fragments form unique patterns‚ which help to distinguish the base for DNA identification. This lab answers the question “whose DNA was left behind?”. Materials: * Transfer pipets * Agarose Gel * Dyed DNA samples *

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    The picture above shows a typical gel electrophoresis set up. The clear container in the center of the picture is called a gel electrophoresis chamber. It contains the agarose gel that will be loaded with genetic material‚ as well as a buffer solution. It is connected to a DC power supply via electrodes. This picture was taken at Paw Print Genetics laboratory in Spokane‚ Washington. Viney and Fenton (1998) defined the term electrophoresis as‚ “the migration of charged particles through a static medium

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    Gel Electrophoresis Adventure     Intro  The final goal of this lab was to successfully measure the size of different samples of  DNA by placing each sample into a well in agarose gel and running a current through a  charged chamber. The DNA samples will move through the gel towards the positive charge.  Ideally‚ the DNA will move and create and sequence of smallest to largest. This lab exposes  us to DNA technology.     Backround  Gel electrophoresis is used to separate macromolecules like DNA or RNA by size or 

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    the gel after electrophoresis. Gel 1 Gel 2 Lane 7. This is Maddie’s (MCB) sample. Gel 2 Lane 6. This is Madi’s (MN) sample. From our sample of the gel electrophoresis‚ both Madi and me are homozygous positive (+/+) for the Alu gene. This can be determined by looking at the ladder and comparing our sample to it‚ to find out if we are homozygous or heterozygous. Discussion For this lab‚ DNA from our cheek cells were separated through PCR‚ and singled out through gel electrophoresis

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