16 research outputs found
Change of the closeness between students by cross-age interaction in elementary school
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Sense-antisense TIN transcript pairs simultaneously detected at different ranges of signal intensities for each of three different tissues
No full text<p><b>Copyright information:</b></p><p>Taken from "Genome mapping and expression analyses of human intronic noncoding RNAs reveal tissue-specific patterns and enrichment in genes related to regulation of transcription"</p><p>http://genomebiology.com/2007/8/3/R43</p><p>Genome Biology 2007;8(3):R43-R43.</p><p>Published online 26 Mar 2007</p><p>PMCID:PMC1868932.</p><p></p> The percentages of TIN transcript pairs simultaneously transcribed from the same genomic locus in both the sense and antisense orientations (full symbols), and detected at different ranges of signal intensities, are shown for each of three different tissues: liver (diamonds), prostate (triangles) and kidney (squares). The percentages of TIN messages transcribed in each tissue from only one of the two DNA strands (sense or antisense) are shown as open symbols
Frequency of exon skipping and abundance of wholly intronic noncoding transcription in RefSeq genes
No full text<p><b>Copyright information:</b></p><p>Taken from "Genome mapping and expression analyses of human intronic noncoding RNAs reveal tissue-specific patterns and enrichment in genes related to regulation of transcription"</p><p>http://genomebiology.com/2007/8/3/R43</p><p>Genome Biology 2007;8(3):R43-R43.</p><p>Published online 26 Mar 2007</p><p>PMCID:PMC1868932.</p><p></p> Distribution of exon skipping events along spliced RefSeq genes with 7, 8, 9 or 10 exons. Filled squares indicate the average frequency of skipping per exon for genes with evidence of TIN RNAs mapping to their introns. Open squares indicate the average frequency of skipping per exon for genes with no evidence in GenBank that TIN RNAs map to their introns. A significantly higher (< 0.002) frequency of exon skipping was observed for RefSeq genes with TIN RNA transcription. Distribution of TIN transcripts among the introns of RefSeq sequences with 7, 8, 9 or 10 introns selected from GenBank as being outside the 95% confidence level of significance (not correlated) in a Pearson correlation analysis between the abundance of TIN contigs per intron and the intron size (in nt). Bars indicate the average intron size (nt) for this selected set of genes. Triangles indicate the number of TIN contigs per intron for RefSeq genes for the same set
Effect of RNAP II inhibitor α-amanitin on the abundance of protein-coding, antisense TIN, sense TIN and antisense PIN RNAs
No full text<p><b>Copyright information:</b></p><p>Taken from "Genome mapping and expression analyses of human intronic noncoding RNAs reveal tissue-specific patterns and enrichment in genes related to regulation of transcription"</p><p>http://genomebiology.com/2007/8/3/R43</p><p>Genome Biology 2007;8(3):R43-R43.</p><p>Published online 26 Mar 2007</p><p>PMCID:PMC1868932.</p><p></p> Lines on each panel represent various transcripts for which the expression levels differed significantly between α-amanitin-treated prostate cells and untreated control cells. Each sample replica is shown in one column. Transcripts were selected by a SAM two-class test (FD
Design and overall performance of the 44 k gene-oriented intron-exon expression oligoarray
No full text<p><b>Copyright information:</b></p><p>Taken from "Genome mapping and expression analyses of human intronic noncoding RNAs reveal tissue-specific patterns and enrichment in genes related to regulation of transcription"</p><p>http://genomebiology.com/2007/8/3/R43</p><p>Genome Biology 2007;8(3):R43-R43.</p><p>Published online 26 Mar 2007</p><p>PMCID:PMC1868932.</p><p></p> Schematic view of the 44 k combined intron-exon expression oligoarray 60-mer probe design. Probe 1 is for the antisense PIN transcripts (blue arrow). Probes 3 and 4 are a pair of reverse complementary sequences designed to detect antisense or sense TIN transcripts (black and hashed black arrows, respectively) in a given locus. Sense exonic probes 2 and 5 are for the protein-coding transcripts (red block and red arrow). Note that the latter were not systematically designed for an exon near the TIN message; in most instances a distant, 3' exon of the gene has been probed instead. Average signal intensity distribution for antisense TIN (solid black line), sense TIN (dashed line), antisense PIN (blue line), or sense protein-coding exonic (red line) probes. Average intensities from six different hybridization experiments with three different human tissues, namely liver, prostate and kidney, are shown. Only probes with intensities above the average negative controls plus 2 SD were considered. The average intensity distribution for probes below this low-limit detection cutoff is shown in the curve marked as 'Not expressed RNAs' (gray line)
Expression signatures of wholly intronic RNAs relative to their 3' protein-coding exons
No full text<p><b>Copyright information:</b></p><p>Taken from "Genome mapping and expression analyses of human intronic noncoding RNAs reveal tissue-specific patterns and enrichment in genes related to regulation of transcription"</p><p>http://genomebiology.com/2007/8/3/R43</p><p>Genome Biology 2007;8(3):R43-R43.</p><p>Published online 26 Mar 2007</p><p>PMCID:PMC1868932.</p><p></p> Cross-referencing of the tissue signatures shown in Figure 10 identified subsets of TIN RNAs that have correlated patterns of expression relative to the 3' protein-coding exon signature from the corresponding genomic loci: 38 pairs were identified in which the 3' exon of the protein-coding transcript (right panel) follows a similar expression pattern to that of the antisense TIN RNA (left panel); 16 pairs were identified in which the 3' exon of the protein-coding transcript (right panel) follows a pattern of tissue expression inverted in relation to that of the antisense TIN RNA (left panel); 64 pairs were identified in which the 3' exon of the protein-coding transcript (right panel) follows a similar expression pattern as that of the sense TIN RNA (left panel); 22 pairs were identified where the 3' exon of the protein-coding transcript (right panel) follows a pattern of tissue expression inverted in relation to that of the sense TIN RNA (left panel). For each line in each panel, expression intensities among the three tissues were normalized within each type of probe and colored as a function of the number of standard deviations from the mean value
Expression signatures of antisense PIN RNAs and corresponding PIN RNA-overlapped exon pairs relative to their 3' protein-coding exons
No full text<p><b>Copyright information:</b></p><p>Taken from "Genome mapping and expression analyses of human intronic noncoding RNAs reveal tissue-specific patterns and enrichment in genes related to regulation of transcription"</p><p>http://genomebiology.com/2007/8/3/R43</p><p>Genome Biology 2007;8(3):R43-R43.</p><p>Published online 26 Mar 2007</p><p>PMCID:PMC1868932.</p><p></p> A subset of 64 pairs of antisense PIN RNAs and corresponding PIN RNA-overlapped exons were identified among the tissue signatures shown in Figure 10 as having correlated patterns of expression: 49 pairs were identified in which the 3' exon of the protein-coding transcript (right panel) follows a similar expression pattern to that of the PIN RNA/PIN RNA-overlapped exon pair (left and central panels); 9 pairs were identified in which the 3' exon of the protein-coding transcript (right panel) does not follow the pattern of tissue expression of the PIN RNA and the corresponding PIN RNA-overlapped exon (left and central panels); 6 pairs in which the PIN RNA (left panel) has an expression pattern inverted in relation to that of the PIN RNA-overlapped exon (central panel). Each line represents a genomic locus covered by three different types of probes (antisense PIN RNA, PIN RNA-overlapped protein-coding exon and 3' protein-coding exon). For each line, expression intensities among the three tissues were normalized within each type of probe and colored as a function of the number of standard deviations from the mean value
