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SDSPAGE异常电泳现象及分析
2006-4 raimi 编辑整理 於 DICP
SDSHall of Shame
You may very well have prepared a nearly perfect gel, and would have a difficult time improving
upon the product. If that is so, then by all means gloat about it! If you didnt do such a hot job dont
despair. All good scientists learn from their mistakes, in fact, without making mistakes most of us
wouldnt learn much at all!
The Hall of Shame presents examples of some of the worst gels students (and instructor) have
run in past labs, with an example or two from a research lab. They represent many of the ways one
can mess up a gel (but not all of them - were still finding new ways!). See what features of your
own gel(s) were unsatisfactory - or at least less than perfect - and use the illustrations to figure out
what you might do to improve your technique.
To critique your own work identify your symptoms and use the gallery to select appropriate
example(s). Each example is linked to a full sized image with suggessted explanations for the
symptoms. From this hall of shame you should be able to determine what can be done to correct
the problem(s). If you wish you may browse by descriptions of symptoms, listed below the gallery.
Symptoms 1—Smears
Smeared gels – example 1
Smearing can have a variety of causes, but most commonly it is due to an unevenly poured acrylamide mixture
or due to gross overloading of protein.
In this example the gel was not properly poured, so that the lower half had begun to polymerize before the upper
part was poured. The first gel mix began to polymerize too quickly. Rather than prepare a new gel cassette, the
students simply stopped pouring, prepared a new mix, and poured it on top of the old. Obviously, the bond wasnt
particularly good.
Smeared gels – example 2
In this example a lot of protein was loaded in each of the wells, all the way across.
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