| 2D gels for protein separation |
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| originally an analytic tool; increasing a preparative tool |
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| separate proteins according to isoelectric point and mass |
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| can overload gels, use narrow pH ranges, do prior |
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| fractionation,… |
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| visible spots are biased towards highly expressed proteins; do |
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| badly on membrane proteins, highly acidic/basic proteins |
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| without special preparative steps |
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