This document describes the procedures for extracting total RNA from post-mortem human brain tissue, synthesizing cDNA from the extracted RNA, and performing semi-quantitative PCR to measure dopamine transporter (DAT) mRNA levels relative to the housekeeping gene cyclophilin. Total RNA is extracted from frozen brain tissue samples using guanidinium thiocyanate-phenol-chloroform extraction. First-strand cDNA is then synthesized from the extracted RNA using oligo-dT primers and Superscript II reverse transcriptase. Semi-quantitative PCR is performed to amplify DAT and cyclophilin cDNA using gene-specific primers, with cyclophilin used to normalize DAT mRNA levels between samples.
This document describes the procedures for extracting total RNA from post-mortem human brain tissue, synthesizing cDNA from the extracted RNA, and performing semi-quantitative PCR to measure dopamine transporter (DAT) mRNA levels relative to the housekeeping gene cyclophilin. Total RNA is extracted from frozen brain tissue samples using guanidinium thiocyanate-phenol-chloroform extraction. First-strand cDNA is then synthesized from the extracted RNA using oligo-dT primers and Superscript II reverse transcriptase. Semi-quantitative PCR is performed to amplify DAT and cyclophilin cDNA using gene-specific primers, with cyclophilin used to normalize DAT mRNA levels between samples.
This document describes the procedures for extracting total RNA from post-mortem human brain tissue, synthesizing cDNA from the extracted RNA, and performing semi-quantitative PCR to measure dopamine transporter (DAT) mRNA levels relative to the housekeeping gene cyclophilin. Total RNA is extracted from frozen brain tissue samples using guanidinium thiocyanate-phenol-chloroform extraction. First-strand cDNA is then synthesized from the extracted RNA using oligo-dT primers and Superscript II reverse transcriptase. Semi-quantitative PCR is performed to amplify DAT and cyclophilin cDNA using gene-specific primers, with cyclophilin used to normalize DAT mRNA levels between samples.
This document describes the procedures for extracting total RNA from post-mortem human brain tissue, synthesizing cDNA from the extracted RNA, and performing semi-quantitative PCR to measure dopamine transporter (DAT) mRNA levels relative to the housekeeping gene cyclophilin. Total RNA is extracted from frozen brain tissue samples using guanidinium thiocyanate-phenol-chloroform extraction. First-strand cDNA is then synthesized from the extracted RNA using oligo-dT primers and Superscript II reverse transcriptase. Semi-quantitative PCR is performed to amplify DAT and cyclophilin cDNA using gene-specific primers, with cyclophilin used to normalize DAT mRNA levels between samples.
Download as DOCX, PDF, TXT or read online from Scribd
Download as docx, pdf, or txt
You are on page 1of 3
one, UK ; Ž .
PhosphoImagere:SF model 455 and ImageQuant Ž . e
Ž . software version 3.3 were from Molecular Dynamics Ž . Sunnyvale, CA, USA . 3.2. Chemicals and reagents Superscript II preamplification system for first strand cDNA synthesis, oligonucleotide primers, Taq DNA polymerase, dNTPs, T7 RNA polymerase, RNasin, RNase free RQ1 DNase were from Gibco BRL Life Technologies; RNA century marker plus template was from Ambion Ž . Austin, TX, USA ; wa- P -dCTP 3000 Ci 32 x Ž rmmol, 10 mCirml was from Dupont NEN Boston, MA, USA ; . Ž . sodium lauryl sarcosinate, guanidinium thiocyanate, phenol, isoamyl alcohol, chloroform, formamide, xylene Žcyanol, sodium pyrophosphate were from Sigma St. Louis,. MO, USA . 3.3. Brain tissue preparation Post-mortem human brain specimens were obtained at routine autopsy from drug-free, age-matched control subjects Ž . Ns8; 32.1"2.8 years; six males; two females . The brain was photographed and cut into 1.5 cm coronal slabs. We fabricated a plexiglass holder with guide plates at 1 cm intervals to facilitate whole-brain sectioning. The anterior and posterior aspects of each block were photographed to record sulcal patterns and structural landmarks. The coronal blocks were rapidly frozen in 2-methylbutane on dry ice at y308C and were subsequently stored at y708C. The post mortem interval ranged between 8 to 27 h average 15.8 Ž . "2.3, mean"S.E. . The substantia nigra was dissected from cryopreserved coronal block specimens taken at a level through the posterior commisure, the medial and lateral geniculate bodies, and the red nucleus. ŽA series of three small lateral to medial punches 200 mg. wet weight were pooled from the pars compacta of the A9 dopaminergic cell group. 4. Detailed procedure The semi-quantitative RT-PCR approach shown here is modified from the common co-amplification method, which was first developed by Chelly et al. 5 . The method shown w x here uses separate amplification of a marker gene along with the target of interest. The constitutively expressed housekeeping gene cyclophilin was used to normalize the level of DAT mRNA. This approach afforded a direct comparison of DAT mRNA levels in reference to cyclophilin expression to be made across individual control subjects. 4.1. Total RNA extraction from human brain tissue Total RNA was prepared from cryopreserved human brain specimen 7,20 . Using oligo dT primers, mR- w x Ž .12 – 18 NAs in 5 mg of total RNA was specifically reverse transcribed and later amplified for studying the relative mRNA levels in different samples. To ensure the lack of contamination of the RNA preparation with genomic DNA, it is recommended to pretreat the RNA samples with RNase-free DNase I. The detailed procedure involves the following steps. Ž . a Weigh the frozen brain tissue punches and prepare the homogenization solution, which contained 4 M guanidium thiocyanate, 25 mM sodium citrate, 0.5% v Ž . rv sarcosyl and 0.72% v Ž . rv b-mercaptoethanol. Ž . Ž . b Add 10 volumes ml of the homogenization solution v Ž . rv to the brain tissue according to the weight of the brain sample mg and homogenize with a Brinkmann Ž . polytron homogenizer for 15 s at a setting of 2.5. Ž . c Mix the solution thoroughly by inverting the tube 10 times after the addition of each of the following reagents: 0.1 volume of the tissue weight of 3 M sodium acetate, Ž . pH 5.2, 1 volume of the wet brain tissue weight of water Ž . saturated phenol, and 0.2 volume of chloroform:isoamyl alcohol 49:1 mixture. Vortex the mix vigorously for 10 s Ž . and chill on ice for 15 min. Ž . d Separate the organic and aqueous phases by centrifugation Sorvall HS-4 rotor, 5.75 cm radius at 6500 Ž . rpm at 48C for 20 min. Transfer the RNA-containing aqueous phase carefully into a fresh centrifuge tube, and precipitate the RNA by addition of an equal volume of cold isopropanol. Store sample at y808C for at least 1 h and then centrifuge Sorvall SS-34 rotor at 15,000 rpm, Ž . 48C for 20 min to pellet RNA. Ž . e Aspirate the supernatant and dissolve the RNA pellet in 0.15–0.2 ml of the homogenization solution, and transfer it to a 1.5 ml Eppendorf tube. Precipitate RNA again by the addition of 2.5 volumes v Ž . rv of cold ethanol and chill at y808C for at least 1 h. Centrifuge the solution for 20 min at 48C in a Brinkmann eppendorf centrifuge Ž . Ž . model 5415 at maximum speed 14,000=g and wash the pellet with 1 ml of cold 75% ethanol. Ž . f Briefly dry the pellet and dissolve in 10 ml of Tris EDTA buffer 10 mM Tris, pH 8.0, 1 mM EDTA , Ž . followed by addition of 1 ml of RNase-free RQ1 DNase for digestion at 37FC for 1 h. Add 40 ml of Tris EDTA buffer and extract with equal volume of phenol:chloroform:isoamyl alcohol 25:24:1 twice. Precipitate RNA by Ž . adding 5 ml of 3 M ammonium acetate pH 5.2 , 125 Ž . ml of ethanol and store at y808C for 1 h. Ž . g Centrifuge for 10 min at the speed of 14,000=g in a microcentrifuge, followed by one wash with 1 ml of 70% 134 L. Chen et al.rBrain Research Protocols 4 1999 132–139 ( ) ethanol. Briefly dry the RNA pellet under vacuum. Resuspend the pellet in 20–30 ml of Tris–EDTA pH 8.0 , and Ž. quantitation by absorbance Ž . A reading at 260 nm and 280 nm. The final preparation should be free of protein with the A260 280 rA ratios across runs at 1.8 or higher. 4.2. First strand cDNA synthesis The first strand synthesis was accomplished by using the Superscript II Preamplification System for First Strand cDNA Synthesis kit from Gibco BRL. The cDNA protocol includes the following steps. Ž . Ž . a Add 1 ml of oligo dT primer 100 pmol to 5 12 – 18 mg of total RNA sample and make the final volume to 12 ml by addition of diethylpyrocarbonate DEPC treated Ž . H O. Incubate at 70 2 8C for 10 min, followed by chill on ice for at least 1 min. Ž . b Prepare a master reaction mix according to the total number of reactions Ž . n , including one no-RT reaction and Žone control RT reaction use a known RNA template. provided in the kit . Therefore, the mix contains n=2 ml of 10=PCR buffer, n=2 ml of 25 mM MgCl , 2 n=1 ml of deoxynucleoside triphosphate dNTP mix and Ž . n=2 ml of 0.1 M dithiothreitol DTT . Add 7 Ž . ml of the above mixture to each sample and mix the solution well, followed by a brief centrifugation step. Ž . c Incubation of the above solution for 5 min at 428C, and then add 1 ml of superscript II Reverse Transcriptase to each tube for the no RT control, substitute 1 Ž ml of DEPC-treated H O . Incubate for 50 min at 42 2 . 8C and then terminate the reaction by incubation at 708C for 15 min, followed by chilling on ice. Briefly centrifuge and then add 1 ml of RNase H to remove the residual RNAs and incubate for 20 min at 378C. Store the samples at y208C. 4.3. Polymerase chain reaction The protocol described here is provided as an example of a general method and uses the constitutively expressed cyclophilin mRNA as an internal control of the semiquantitative PCR to measure DAT mRNA in human substantia nigra that was regionally dissected from post mortem brains of drug-free and age-matched male and female subjects. DAT and cyclophilin primers were created using PrimerDesign software version 1.10, Marburg, Germany Ž . with similar GC content 50–60% and melting tempera- Ž . ture Ž . Tm 55–608C . The specificity of the primers was later confirmed by southern hybridization with an in vitro synthesized radiolabeled human DAT or cyclophilin probe for the amplified fragments, respectively. These primers do not span any intron regions since they anneal to the cDNAs that were reverse transcribed from mRNAs. The primers were synthesized by Gibco BRL Life Technologies according to manufacturer’s instructions Table 1 .