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One of the most problematic steps in RNA isolation
is the first step - thorough lysis of the tissue or cell sample in
a denaturant solution that inhibits RNA degradation by RNase. While
it is possible to process fresh tissue directly, it is extremely
important that all cells are disrupted immediately upon contact with
the denaturant. This usually requires use of a polytron and even
then some "difficult to process tissues" (e.g. hard tumors,
bacterial cells, plant roots, etc.) are not effectively disrupted
(see the article, "Cell Disruption:
Getting the RNA Out "). Therefore, if you are having a problem
with yield or degradation during RNA isolation, we usually recommend
freezing the tissue sample before processing. Here we compare three
methods for processing frozen tissues in a side-by-side test for
quantity of mRNA recovered.
Freezing the Tissue
Samples should be frozen quickly so that
the whole tissue sample freezes at once throughout. This may mean
mincing the tissue into smaller fragments before freezing. Submerging
the samples in liquid nitrogen will freeze the tissue pieces most
quickly. Alternatively, a metal plate placed on dry ice can serve
as a freezing surface.
Each of the methods below describes a distinct
way of generating a tissue/cell lysate from which to purify RNA
and is assessed for yield of poly(A+)RNA, when used to process
0.1 g of frozen mouse liver tissue. While the three methods each
use a guanidine buffer to ultimately lyse the cells, they differ
in how the tissue is processed prior or during that lysis step.
Method 1: Processing frozen tissue fragments
in a dounce
Yield: 4.1 µg poly(A+)RNA
Frozen tissue is cut into small pieces (approx.
0.5 cm2) on dry ice, placed in a dounce, and processed as
lysis buffer is added. Both pestle A and pestle B are used for ten strokes
each.
Method 2: Processing frozen tissue fragments
through a syringe
Yield: 3.2 µg poly(A+)RNA
Frozen tissue is cut into small pieces
(approx. 0.5 cm2) on dry ice, added
to lysis buffer and passed back and forth ten times through an 18
gauge syringe needle.
Method 3: Grinding the tissue to a powder in
liquid N2
Yield: 7.1 µg poly(A+)RNA
The frozen sample is powdered by grinding
the frozen tissue fragments in a prechilled mortar and occasionally
adding liquid N2 into the mortar
to prevent thawing. Once the tissue is ground to a fine powder, the
denaturing solution is added to the mortar, and the semi-frozen mixture
is stirred. This mixture can then be thawed and transferred to an
appropriate vessel for further processing.
Note that by grinding the tissue to a powder
in liquid N2 (Method 3), cellular disruption is much
more complete resulting almost twice the yield of the other two
methods.
Reprinted from Ambion's TechNotes
Newsletter 3:3, © 1998
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