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miRNA array or deep sequencing
3Â¥2009-12-25 21:32:43
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telomerase

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Somatodendritic microRNAs identified by laser capture and multiplex RT-PCR

Access the most recent version at doi:10.1261/rna.480407
RNA 2007 13: 1224-1234 originally published online June 25, 2007
Min-Jeong Kye, Tsunglin Liu, Sasha F. Levy, et al.
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4Â¥2009-12-26 03:49:57
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telomerase

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chuang1381(½ð±Ò+3,VIP+0): 1-5 17:52
Real-time RT-PCR for miRNA detection
187-plex RT-PCR was adapted for the rat sequences from Lao
et al. (2006) based on Sanger¡¯s October 2005 registry. Briefly,
multiplex reverse transcription primers were generated with a
common 20-nt stem¨Cloop followed by 8 nt complementary to
the 39-end of a given miRNA (e.g., 59-AACTATAC-39 for rnolet-
7a). Reverse transcriptase reactions were performed in 5 mL
containing 13 cDNA Archiving Kit buffer (Applied Biosystems),
10 units of MMLV reverse transcriptase, 1.25 mM each dNTP,
1.3 units of RNase inhibitors (Applied Biosystems), 2.5 nM each
reverse primer, and 2 mL of laser capture microdissection samples.
Reactions were 30 cycles for 30 sec at 20¡ãC, 30 sec at 42¡ãC, and
1 sec at 50¡ãC and one cycle for 5 min at 85¡ãC to inactivate the
enzyme.
Pre-PCR
cDNA was pre-amplified using a common reverse primer (UR) to
the 20-nt stem¨Cloop and multiplexed z18-nt forward primers
(FPs) with a common 59-end and a 39-end matching 12¨C17 nt of
the 59-end of a given miRNA (e.g., 59-TCCAGCTCCTATATGAT-
39 for rno-let-7a). The amplification was performed in 25 mL
containing 13 Universal Master Mix with no UNG (Applied
Biosystems), 50 nM each FP, 5 mM UR, 6.25 units of AmpliTaq
Gold polymerase (Applied Biosystems), 0.5 mM each dNTP,
2 mM MgCl2, and 5 mL of the initial reverse transcriptase amplification.
Reactions were one cycle of 10 min at 95¡ãC, 2 min at
55¡ãC, and 14 cycles of 1 sec at 95¡ãC and 1 min at 65¡ãC.
Real-time PCR
The product of this amplification was diluted four times, and
0.1 mL was used for real-time PCR performed in 10 mL containing
13 Universal Master Mix with no UNG (Applied Biosystems),
0.25 mM FP, 0.1 mM TaqMan probe, and 5 mM UR. The miRNA
specificity for each reaction was provided by the miRNA-specific
sequences of the FP and TaqMan probes. Real-time PCR was
performed in a Biosystems 7500HT 96-well plate Sequence Detection
System using 40 cycles of 15 sec at 95¡ãC and 1 min at 60¡ãC.
All reactions were run in duplicate. The threshold cycle (Ct)
was determined as the fractional cycle number at which the
fluorescence passes the fixed threshold. For primer sequences, see
Supplemental Table 2. All Ct values were averaged over two to
four repeated biological experiments each with two averaged realtime
PCR experimental replicates.
Single-plex real-time PCR
Single-plex real-time PCR was performed as described for multiplex
real-time PCR with one modification: A single miRNAspecific
primer was used instead of multiple primers.
Real-time PCR for mRNA detection
RT-PCR was performed to measure the amount of mRNAs in the
same laser capture microdissected samples. Reverse transcriptase
reactions were performed in 5 mL containing 13 cDNA Archiving
Kit buffer (Applied Biosystems), 10 units MMLV reverse transcriptase,
1.25 mM each dNTP, 1 unit of RNase inhibitor (Applied
Biosystems), 2 mM random primer, and 1 mL of laser capture
microdissection samples. Reactions were 10 min at 20¡ãC, 120 min
at 37¡ãC, and 5 min at 85¡ãC to inactivate the enzyme. cDNA was
pre-amplified using gene-specific forward primers and reverse
primers. The amplification was performed in 25 mL containing
13 Universal Master Mix with no UNG (Applied Biosystems),
50 nM each FP, 50 nM each RP, 6.25 units of AmpliTaq Gold
polymerase (Applied Biosystems), 0.5 mM each dNTP, 0.75 mM
MgCl2, and 5 mL of the initial reverse transcriptase amplification.
Reactions were one cycle for 10 min at 95¡ãC, 2 min at 55¡ãC, and
14 cycles of 1 sec at 95¡ãC and 1 min at 65¡ãC. The product of this
amplification was diluted four times, and 0.1 mL was used for realtime
PCR reactions detecting mRNAs. It was performed in 10 mL
coBiosystems), 500 nM FP, 200 nM TaqMan probe, and 500 nM UR.
Real-time PCR was performed as above. For primer sequences, see
Supplemental Table 1.ntaining 13 Universal Master Mix with no UNG (Applied
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5Â¥2009-12-26 03:52:20
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