Electrophoresis

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This article is currently being developed as part of an Eduzendium student project in the framework of a course entitled BEE 4640 Bioseparation Processes at Cornell University. The course homepage can be found at CZ:Cornell_University_2010_BEE_4640_Bioseparation_Processes.
For the course duration, the article is closed to outside editing. Of course you can always leave comments on the discussion page. The anticipated date of course completion is 21 December 2010. One month after that date at the latest, this notice shall be removed.
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Note to course participants: Looking forward to some insightful and useful articles from your collaborations.


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Electrophoresis is a separation technique frequently used in the analysis of proteins and nucleic acids. The process known as electrophoresis, involves the migration of particles or molecules (in particular proteins, DNA, and RNA) through an electric field that separates them exclusively on the basis of their size or molecular weight. The direction the molecule moves depends on its charge while the rate of migration is affected by the size, shape, density of the gel and the strength of the applied current (5c). Electrophoresis is a very simple process and relatively quick with a high resolution. In addition electrophoresis is an extremely useful method to estimate the purity of a sample. The technique is also very sensitive to slight variations in molecular weight, size, and even shape of nucleic acids and proteins (1). Electrophoresis can also be useful when it doesn’t affect the molecule’s structure or denature the protein (1).

The Process

Here, go into more detail about the process.

History

This section should describe the invention and development of the process. If the section runs long, divide it into chronological subsections, for example:

Invention and early development

This subsection should provide some historical context for the development of your process, describe its invention, and name some early developers and/or applications.

Recent developments

This section should discuss new developments in the field. Don't hesitate to drop in brief mentions of processes or features you don't intend to discuss in depth. By so doing you are planting seeds of articles which will eventually be developed by others.[1]

Design and Operation

Use lots of subsections here as you describe various aspects of the process .[2]

Applications

This section should discuss how the process is used in practice.[3]

Examples

If you have used a lot of equations in your article, this may be a good place to show an example of how they are used. See the article on the Antoine Equation for an example.


All unapproved Citizendium articles may contain errors of fact, bias, grammar etc. A version of an article is unapproved unless it is marked as citable with a dedicated green template at the top of the page, as in this version of the 'Biology' article. Citable articles are intended to be of reasonably high quality. The participants in the Citizendium project make no representations about the reliability of Citizendium articles or, generally, their suitability for any purpose.

Attention niels epting.png
Attention niels epting.png
This article is currently being developed as part of an Eduzendium student project in the framework of a course entitled BEE 4640 Bioseparation Processes at Cornell University. The course homepage can be found at CZ:Cornell_University_2010_BEE_4640_Bioseparation_Processes.
For the course duration, the article is closed to outside editing. Of course you can always leave comments on the discussion page. The anticipated date of course completion is 21 December 2010. One month after that date at the latest, this notice shall be removed.
Besides, many other Citizendium articles welcome your collaboration!

Note to course participants: Looking forward to some insightful and useful articles from your collaborations.


This article is a stub and thus not approved.
Main Article
Discussion
Related Articles  [?]
Bibliography  [?]
External Links  [?]
Citable Version  [?]
 
This editable Main Article is under development and subject to a disclaimer.

Electrophoresis is a separation technique frequently used in the analysis of proteins and nucleic acids. The process known as electrophoresis, involves the migration of particles or molecules (in particular proteins, DNA, and RNA) through an electric field that separates them exclusively on the basis of their size or molecular weight. The direction the molecule moves depends on its charge while the rate of migration is affected by the size, shape, density of the gel and the strength of the applied current (5c). Electrophoresis is a very simple process and relatively quick with a high resolution. In addition electrophoresis is an extremely useful method to estimate the purity of a sample. The technique is also very sensitive to slight variations in molecular weight, size, and even shape of nucleic acids and proteins (1). Electrophoresis can also be useful when it doesn’t affect the molecule’s structure or denature the protein (1).

The Process

Here, go into more detail about the process.

History

This section should describe the invention and development of the process. If the section runs long, divide it into chronological subsections, for example:

Invention and early development

This subsection should provide some historical context for the development of your process, describe its invention, and name some early developers and/or applications.[4]

Recent developments

This section should discuss new developments in the field. Don't hesitate to drop in brief mentions of processes or features you don't intend to discuss in depth. By so doing you are planting seeds of articles which will eventually be developed by others.[5]

Design and Operation

Use lots of subsections here as you describe various aspects of the process .[6]

Applications

This section should discuss how the process is used in practice.[7]

Examples

If you have used a lot of equations in your article, this may be a good place to show an example of how they are used. See the article on the Antoine Equation for an example.


All unapproved Citizendium articles may contain errors of fact, bias, grammar etc. A version of an article is unapproved unless it is marked as citable with a dedicated green template at the top of the page, as in this version of the 'Biology' article. Citable articles are intended to be of reasonably high quality. The participants in the Citizendium project make no representations about the reliability of Citizendium articles or, generally, their suitability for any purpose.

Attention niels epting.png
Attention niels epting.png
This article is currently being developed as part of an Eduzendium student project in the framework of a course entitled BEE 4640 Bioseparation Processes at Cornell University. The course homepage can be found at CZ:Cornell_University_2010_BEE_4640_Bioseparation_Processes.
For the course duration, the article is closed to outside editing. Of course you can always leave comments on the discussion page. The anticipated date of course completion is 21 December 2010. One month after that date at the latest, this notice shall be removed.
Besides, many other Citizendium articles welcome your collaboration!

Note to course participants: Looking forward to some insightful and useful articles from your collaborations.


This article is a stub and thus not approved.
Main Article
Discussion
Related Articles  [?]
Bibliography  [?]
External Links  [?]
Citable Version  [?]
 
This editable Main Article is under development and subject to a disclaimer.

Electrophoresis is a separation technique frequently used in the analysis of proteins and nucleic acids. The process known as electrophoresis, involves the migration of particles or molecules (in particular proteins, DNA, and RNA) through an electric field that separates them exclusively on the basis of their size or molecular weight. The direction the molecule moves depends on its charge while the rate of migration is affected by the size, shape, density of the gel and the strength of the applied current (5c). Electrophoresis is a very simple process and relatively quick with a high resolution. In addition electrophoresis is an extremely useful method to estimate the purity of a sample. The technique is also very sensitive to slight variations in molecular weight, size, and even shape of nucleic acids and proteins (1). Electrophoresis can also be useful when it doesn’t affect the molecule’s structure or denature the protein (1).

The Process

Here, go into more detail about the process.

History

This section should describe the invention and development of the process. If the section runs long, divide it into chronological subsections, for example:

Invention and early development

This subsection should provide some historical context for the development of your process, describe its invention, and name some early developers and/or applications.[8]

Recent developments

This section should discuss new developments in the field. Don't hesitate to drop in brief mentions of processes or features you don't intend to discuss in depth. By so doing you are planting seeds of articles which will eventually be developed by others.[9]

Design and Operation

Use lots of subsections here as you describe various aspects of the process .[10]

Applications

This section should discuss how the process is used in practice.[11]

Examples

If you have used a lot of equations in your article, this may be a good place to show an example of how they are used. See the article on the Antoine Equation for an example.


All unapproved Citizendium articles may contain errors of fact, bias, grammar etc. A version of an article is unapproved unless it is marked as citable with a dedicated green template at the top of the page, as in this version of the 'Biology' article. Citable articles are intended to be of reasonably high quality. The participants in the Citizendium project make no representations about the reliability of Citizendium articles or, generally, their suitability for any purpose.

Attention niels epting.png
Attention niels epting.png
This article is currently being developed as part of an Eduzendium student project in the framework of a course entitled BEE 4640 Bioseparation Processes at Cornell University. The course homepage can be found at CZ:Cornell_University_2010_BEE_4640_Bioseparation_Processes.
For the course duration, the article is closed to outside editing. Of course you can always leave comments on the discussion page. The anticipated date of course completion is 21 December 2010. One month after that date at the latest, this notice shall be removed.
Besides, many other Citizendium articles welcome your collaboration!

Note to course participants: Looking forward to some insightful and useful articles from your collaborations.


This article is a stub and thus not approved.
Main Article
Discussion
Related Articles  [?]
Bibliography  [?]
External Links  [?]
Citable Version  [?]
 
This editable Main Article is under development and subject to a disclaimer.

Electrophoresis is a separation technique frequently used in the analysis of proteins and nucleic acids. The process known as electrophoresis, involves the migration of particles or molecules (in particular proteins, DNA, and RNA) through an electric field that separates them exclusively on the basis of their size or molecular weight. The direction the molecule moves depends on its charge while the rate of migration is affected by the size, shape, density of the gel and the strength of the applied current (5c). Electrophoresis is a very simple process and relatively quick with a high resolution. In addition electrophoresis is an extremely useful method to estimate the purity of a sample. The technique is also very sensitive to slight variations in molecular weight, size, and even shape of nucleic acids and proteins (1). Electrophoresis can also be useful when it doesn’t affect the molecule’s structure or denature the protein (1).

The Process

Here, go into more detail about the process.

History

This section should describe the invention and development of the process. If the section runs long, divide it into chronological subsections, for example:

Invention and early development

This subsection should provide some historical context for the development of your process, describe its invention, and name some early developers and/or applications.[12]

Recent developments

This section should discuss new developments in the field. Don't hesitate to drop in brief mentions of processes or features you don't intend to discuss in depth. By so doing you are planting seeds of articles which will eventually be developed by others.[13]

Design and Operation

Use lots of subsections here as you describe various aspects of the process .[14]

Applications

This section should discuss how the process is used in practice.[15]

Examples

If you have used a lot of equations in your article, this may be a good place to show an example of how they are used. See the article on the Antoine Equation for an example.

References

  1. "New Directions for Flocculation," American Flocculation Society. 2006. Retrieved July 21, 2009 from http://www.amflocsoc.org/future_devs.html
  2. First Author and Second Author, "Electro-absorpto-crossflow-sedimento-extractofractionation," Journal of Superspecialized Bioseparation Arcana 36:2 (2010) pp. 86-52.
  3. "Major Success for Bioprocess Fractionation," Anytown Daily News, January 1, 2015, p. A6.
  4. John Q. Sample, Chromatography, a new analytical tool. City: Publisher, 1885.
  5. "New Directions for Flocculation," American Flocculation Society. 2006. Retrieved July 21, 2009 from http://www.amflocsoc.org/future_devs.html
  6. First Author and Second Author, "Electro-absorpto-crossflow-sedimento-extractofractionation," Journal of Superspecialized Bioseparation Arcana 36:2 (2010) pp. 86-52.
  7. "Major Success for Bioprocess Fractionation," Anytown Daily News, January 1, 2015, p. A6.
  8. John Q. Sample, Chromatography, a new analytical tool. City: Publisher, 1885.
  9. "New Directions for Flocculation," American Flocculation Society. 2006. Retrieved July 21, 2009 from http://www.amflocsoc.org/future_devs.html
  10. First Author and Second Author, "Electro-absorpto-crossflow-sedimento-extractofractionation," Journal of Superspecialized Bioseparation Arcana 36:2 (2010) pp. 86-52.
  11. "Major Success for Bioprocess Fractionation," Anytown Daily News, January 1, 2015, p. A6.
  12. John Q. Sample, Chromatography, a new analytical tool. City: Publisher, 1885.
  13. "New Directions for Flocculation," American Flocculation Society. 2006. Retrieved July 21, 2009 from http://www.amflocsoc.org/future_devs.html
  14. First Author and Second Author, "Electro-absorpto-crossflow-sedimento-extractofractionation," Journal of Superspecialized Bioseparation Arcana 36:2 (2010) pp. 86-52.
  15. "Major Success for Bioprocess Fractionation," Anytown Daily News, January 1, 2015, p. A6.

[1]



(2) Biochem book Nelson, D. L., Cox, M. M. (2008). Lehninger Principles of Biochemistry (5th ed.). New York, NY: W.H. Freeman and Company. a. Online biochem book http://bcs.whfreeman.com/lehninger5e/

(3) Bio lab notes Chen, K., Glase, J. (2009-2010). Chapter 13 – DNA Technology: From Recombination to Genomic Sequencing and Forensic Analysis. In Chen, K. & Hester, L. L. (Eds.), Investigative Biology a laboratory text (pp. 245-288). Plymouth, MI: Hayden McNeil.

(4) Bio online textbook Campbell, N. A., Reece, J. B., Urry, L. A., Cain, M. L., Wasserman, S. A., Minorshky, P. V., et al. (2008). Biology (8th ed.). San Francisco, CA: Benjamin Cummings.

  1. Harrison, R. G., Todd, P., Rudge S. R., Petrides, D. P. (2003). Bioseparations Science and Engineering. New York, NY: Oxford University Press.