RNA Detection

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2.2 In Vitro
Measurement
of Fluorescence
Activation Kinetics



  1. Stopped-flow spectrafluorometer (e.g., Applied Photophysics
    Model SX20).

  2. Spectrofluorophotometer (e.g., Shimazu RF-5300PC).

  3. 50 nM and 0.2μM ECHO-liveFISH probes in PBS.

  4. 0.2, 0.35, 0.7, 1.4, and 2.8μM RNA/DNA single-stranded
    oligonucleotides of targeted sequences in PBS.

  5. Dilution buffer in fluorophotospectral measurement: 4SSC,
    0.5 mM EDTA, 10% dextran sulfate, and 10% deionized form-
    amide in dH 2 O.


2.3 In Vivo
Electroporation



  1. Stereomicroscope.

  2. Micromanipulator (e.g., Narishige MM-3).

  3. Pulse generator (e.g., Nepagene NEPA21).

  4. Tweezer-type cathode electrodes (e.g., Nepagene CUY650P3).

  5. Adaptor cable (e.g., Nepagene C118).

  6. Hook-type anode electrode (e.g., Nepagene C117).

  7. Foot switch (e.g., Nepagene C200).

  8. Injection microsyringe (e.g., ITO Corporation MS-NE05 with
    33-G needle connected to the anode).

  9. Tweezers.

  10. Gauge 27–33 needles.

  11. 70% ethanol.

  12. Sterile ddH 2 O.

  13. 200 ng/μL ECHO-liveFISH probes in TE with 0.1% fast
    green dye.

  14. 3μg/μL DsRed2-B23 expressing DNA plasmids in TE with
    0.1% fast green dye.

  15. 200 ng/μL Cy5-d(T) 30 in TE with 0.1% fast green dye.


2.4 Generating Brain
Slices and Stabilizing
for Fluorescence
Imaging



  1. CO 2 incubator.

  2. Vibratome.

  3. Stereomicroscope mounted with digital camera.

  4. Confocal laser scanning microscope mounted with live-cell
    imaging chamber (e.g., Olympus FV1000).

  5. Temperature and CO 2 control modules.
    6.φ27 mm-hole glass-bottom dish.

  6. Slice anchor.

  7. Artificial cerebrospinal fluid (ACSF):124 mM NaCl, 3 mM
    KCl, 26 mM NaHCO 3 , 2 mM CaCl 2 /2H 2 O, 1 mM
    MgSO 4 /7H 2 O, 1.25 mM KH 2 PO 4 , and 10 mMD-glucose,
    bubbled with a gas mixture of 95% O 2 /5% CO 2 before use.


262 Dan Ohtan Wang

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