From ea46f42ee640928b92947bfb204c41a482d80937 Mon Sep 17 00:00:00 2001 From: root Date: Tue, 8 May 2012 18:39:56 -0500 Subject: Add all the source codes into the github. --- web/dbdoc/HC_M2_1206_R.html | 809 ++++++++++++++++++++++++++++++++++++++++++++ 1 file changed, 809 insertions(+) create mode 100755 web/dbdoc/HC_M2_1206_R.html (limited to 'web/dbdoc/HC_M2_1206_R.html') diff --git a/web/dbdoc/HC_M2_1206_R.html b/web/dbdoc/HC_M2_1206_R.html new file mode 100755 index 00000000..08380605 --- /dev/null +++ b/web/dbdoc/HC_M2_1206_R.html @@ -0,0 +1,809 @@ + +Hippocampus Consortium M430v2(EntrezG_8) December06 RMA + + + + + + + + + + + + + + + + +
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Hippocampus Consortium M430v2(EntrezG_8) December06 RMA +modify this page

Accession number: GN129

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    Summary:

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+PRELIMINARY: The June 2006 Hippocampus Consortium data set provides estimates of mRNA expression in the adult hippocampus of 99 genetically diverse strains of mice including 67 BXD recombinant inbred strains, 13 CXB recombinant inbred strains, a set of diverse inbred strains, and two reciprocal F1 hybrids. + +

The hippocampus is an important and intriguing part of the forebrain that is crucial in memory formation and retrieval, and that is often affected in epilepsy, Alzheimer's disease, and schizophrenia. Unlike most other parts of the brain, the hippocampus contains a remarkable population of stems cells that continue to generate neurons and glial cells even in adult mammals (Kempermann, 2005). This genetic analysis of transcript expression in the hippocampus (dentate gyrus, CA1-CA3) is a joint effort of 14 investigators that is supported by numerous agencies described in the acknowledgments section. + +

Samples were processed using a total of 205 Affymetrix GeneChip Mouse Expression 430 2.0 short oligomer arrays (MOE430 2.0 or M430v2; see GEO platform ID GPL1261), of which 179 passed stringent quality control and error checking . This particular data set was processed using the RMA protocol using a custom CDF. To simplify comparisons among transforms, RMA values of each array were adjusted to an average of 8 units and a standard deviation of 2 units. + + +

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    About the strains used to generate this set of data:

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The BXD genetic reference panel of recombinant inbred strains consists of just over 80 strains. The BXDs in this data set include 27 of the BXD strains made by Benjamin Taylor at the Jackson Laboratory in the 1970s and 1990s (BXD1 through BXD42). All of these strains are fully inbred, many well beyond the 100th filial (F) generation of inbreeding. We have also included 39 inbred (25 strains at F20+) and nearly inbred (14 strains between F14 and F20) BXD lines generated by Lu and Peirce. All of these strains, including those between F14 and F20, have been genotyped at 13,377 SNPs. + +

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Mouse Diversity Panel (MDP). We have profiled a MDP consisting 16 inbred strains and a pair of reciprocal F1 hybrids; B6D2F1 and D2B6F1. These strains were selected for several reasons: +

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  • genetic and phenotypic diversity, including use by the Phenome Project + +
  • their use in making genetic reference populations including recombinant inbred strains, cosomic strains, congenic and recombinant congenic strains +
  • their use by the Complex Trait Consortium to make the Collaborative Cross (Nairobi/Wellcome, Oak Ridge/DOE, and Perth/UWA) +
  • genome sequence data from three sources (NHGRI, Celera, and Perlegen-NIEHS) +
  • availability from The Jackson Laboratory +
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All eight parents of the Collaborative Cross (129, A, C57BL/6J, CAST, NOD, NZO, PWK, and WSB) have been included in the MDP (noted below in the list). Twelve MDP strains have been sequenced, or are currently being resequenced by Perlegen for the NIEHS. This panel will be extremely helpful in systems genetic analysis of a wide variety of traits, and will be a powerful adjunct in fine mapping modulators using what is essentially an association analysis of sequence variants. + +

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  1. 129S1/SvImJ + +
        Collaborative Cross strain sequenced by NIEHS; background for many knockouts; Phenome Project A list + +
  2. A/J +
        Collaborative Cross strain sequenced by Perlegen/NIEHS; parent of the AXB/BXA panel + +
  3. AKR/J +
        Sequenced by NIEHS; Phenome Project B list + +
  4. BALB/cByJ +
        Sequenced by NIEHS; maternal parent of the CXB panel; Phenome Project A list + +
  5. BALB/cJ +
        Widely used strain with forebrain abnormalities (callosal defects); Phenome Project A list + +
  6. C3H/HeJ
        Sequenced by Perlegen/NIEHS; paternal parent of the BXH panel; Phenome Project A list + +
  7. C57BL/6J + +
        Sequenced by NHGRI; parental strain of AXB/BXA, BXD, and BXH; Phenome Project A list + +
  8. C57BL/6ByJ +
        Paternal substrain of B6 used to generate the CXB panel + +
  9. CAST/Ei +
        Collaborative Cross strain sequenced by NIEHS; Phenome Project A list + +
  10. DBA/2J +
        Sequenced by Perlegen/NIEHS and Celera; paternal parent of the BXD panel; Phenome Project A list + +
  11. KK/HlJ +
        Sequenced by Perlegen/NIEHS + +
  12. LG/J +
        Paternal parent of the LGXSM panel + +
  13. NOD/LtJ + +
        Collaborative Cross strain sequenced by NIEHS; Phenome Project B list; diabetic + +
  14. NZO/HlLtJ +
        Collaborative Cross strain + +
  15. PWD/PhJ +
        Sequenced by Perlegen/NIEHS; parental strain for a consomic set by Forjet and colleagues + +
  16. PWK/PhJ +
        Collaborative Cross strain; Phenome Project D list + +
  17. WSB/EiJ
        Collaborative Cross strain sequenced by NIEHS; Phenome Project C list + +
  18. B6D2F1 and D2B6F1 +
    F1 hybrids generated by crossing C57BL/6J with DBA/2J +
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We have not combined data from reciprocal F1s because they have different Y chromosome and mitochondial haplotypes. Parent-of-origin effects (imprinting, maternal environment) may also lead to interesting differences in hippocampal transcript levels. + + +

These strains are available from The Jackson Laboratory. BXD43 through BXD100 strains are available from Lu Lu and colleagues at UTHSC.

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    About the animals and tissue used to generate this set of data:

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BXD animals were obtained from UTHSC, UAB, or directly from The Jackson Laboratory (see Table 1 below). Animals were housed at UTHSC, Beth Israel Deaconess, or the Jackson Laboratory before sacrifice. Virtually all CXB animals were obtained directly at the Jackson Laboratory by Lu Lu. We thanks Muriel Davission for making it possible to collect these cases on site. Standard inbred strain stock was from The Jackson Laboratory, but most animals were housed or reared at UTHSC. Mice were killed by cervical dislocation and brains were removed and placed in RNAlater prior to dissection. Cerebella and olfactory bulbs were removed; brains were hemisected, and both hippocampi were dissected whole by Hong Tao Zhang in the Lu lab. Hippocampal samples are very close to complete (see Lu et al., 2001) but probably include variable amounts of subiculum and fimbria. + +

A pool of dissected tissue typically from six hippocampi and three naive adults of the same strain, sex, and age was collected in one session and used to generate cRNA samples. Two-hundred and one RNA samples were extracted at UTHSC by Zhiping Jia, four samples by Shuhua Qi (R2331H1, R2332H1, P2350H1, R2349H1), and one by Siming Shou (R0129H2). + +

A great majority of animals used in this study were between 45 and 90 days of age (average of 66 days, maximum range from 41 to 196 days; see Table 1 below). +

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Sample Processing: Samples were processed in the INIA Bioanalytical Core at the W. Harry Feinstone Center for Genomic Research, The University of Memphis, led by Thomas R. Sutter. All processing steps were performed by Shirlean Goodwin. In brief, RNA purity was evaluated using the 260/280 nm absorbance ratio, and values had to be greater than 1.8. The majority of samples were 1.9 to 2.1. RNA integrity was assessed using the Agilent Bioanalyzer 2100. We required an RNA integrity number (RIN) of greater than 8. This RIN value is based on the intensity ratio and amplitude of 18S and 28S rRNA signals. The standard Eberwine T7 polymerase method was used to catalyze the synthesis of cDNA template from polyA-tailed RNA using Superscript II reverse transcriptase (Invitrogen Inc.). The Enzo Life Sciences, Inc., BioArray High Yield RNA Transcript Labeling Kit (T7, Part No. 42655) was used to synthesize labeled cRNA. The cRNA was evaluated using both the 260/280 ratio (values of 2.0 or 2.1 are acceptable) and the Bioanalyzer output (a dark cRNA smear on the 2100 output centered roughly between 600 and 2000 nucleotides is required). Those samples that passed both QC steps (10% usually failed and new RNA samples had to be acquired and processed) were then sheared using a fragmentation buffer included in the Affymetrix GeneChip Sample Cleanup Module (Part No. 900371). Fragmented cRNA samples were either stored at -80 deg. C until use or were immediately injected onto the array. The arrays were hybridized and washed following standard Affymetrix protocols. + + +

Replication and Sample Balance: We obtained a male sample pool and female sample pool from each isogenic group. While all strains were orginally represented by matched male and female samples, not all data sets passed the final quality control steps. Seventy-seven of 97 strains are represented by pairs or (rarely) trios of arrays. The first and last samples are technical replicates of a B6D2F1 hippocampal pool (aliquots R1291H3 and R1291H4). + +

Experimental Design and Batch Structure: This data set consists arrays processed in six groups over a three month period (May 2005 to August 2005). Each group consists of 32 to 34 arrays. Sex, strain, and strain type (BXD, CXB, and MDP) were interleaved among groups to ensure reasonable balance and to minimize group-by-strain statistical confounds in group normalization. The two independent samples from a single strain were always run in different groups. All arrays were processed using a single protocol by a single operator, Shirlean Goodwin. + +

All samples in a group were labeled on one day, except for a few cases that failed QC on their first pass. The hybridization station accommodates up to 20 samples, and for this reason each group was split into a large first set of 20 samples and a second set of 12 to 14 samples. Samples were washed in groups of four and then held in at 4 deg C until all 20 (or 12-14) arrays were ready to scan. The last four samples out of the wash stations were scanned directly. Samples were scanned in sets of four. + + +

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    Data Table 1:

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+This table lists all arrays by order of processing (Run), Sample ID, Strain, Sex, Age, number of animals in each sample pool (Pool), F generation number when less than 30 (GenN, and the Source of animals. SampleID is the ID number of the pooled RNA sample with a H1 through H3 suffix to indicate the actual hippocampal RNA aliquot used to prepare cRNA. Grp is the sequential group processing number (1 - 6). + +
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indextube IDstrainagesexbatch IDpool sizelRMA outlierscale factorback ground averagepresentabsentmarginalAFFX-b-ActinMur (3'/5')AFFX-GapdhMur (3'/5')source
1R2028H2129S1/SvImJ66F530.14.36264.490.4970.4840.0192.781.13JAX
2R2029H2129S1/SvImJ66M630.045.20841.210.490.490.021.620.95JAX
3R2670H1A/J65F730.043.95146.80.4980.4850.0171.320.75UTM RW
4R2030H1A/J57M520.063.30745.160.5270.4540.0181.630.99UTM RW
5R2032H3AKR/J66F530.043.05461.030.510.4710.0181.460.79JAX
6R2454H1AKR/J66M640.112.89258.550.4740.5070.0191.990.78JAX
7R1289H2B6D2F164F630.022.40653.840.4920.4890.0191.610.96UTM RW
8R1291H3B6D2F166M130.013.52448.540.4870.4940.0191.211.52UTM RW
9R1291H4B6D2F166M630.083.89146.690.5120.4690.0191.90.89UTM RW
10R1675H1BALB/cByJ83M730.033.40548.130.5090.4740.0181.130.78JAX
11R2036H3BALB/cJ51F530.122.61156.290.5180.4660.0173.31.23UTM RW
12R2053H1BALB/cJ55M530.12.50563.270.4990.4830.0183.11.34UTM RW
13R2037H2BALB/cJ51M640.012.54658.130.4970.4850.0181.260.77UTM RW
14R1507H1BXD158M330.024.05660.170.4780.5030.0191.150.76Glenn
15R1542H1BXD159F730.031.79280.560.4920.4890.0181.570.79Glenn
16R1520H1BXD256F440.091.71571.620.5150.4670.0182.361.6Glenn
17R1516H1BXD261M140.012.23164.860.5080.4740.0191.31.53Glenn
18R1593H2BXD560F1401.91359.960.4870.4930.020.981.44Glenn
19R1692H1BXD560M320.073.76472.740.4650.5160.021.150.74Glenn
20R1539H2BXD659F1402.48854.970.5180.4630.0181.081.33Glenn
21R1538H1BXD659M430.012.58550.270.5050.4750.021.460.79Glenn
22R1518H1BXD856F1302.9254.840.5150.4650.021.321.24Glenn
23R1548H1BXD859M630.072.13259.370.5040.4770.0192.161.54Glenn
24R1350H2BXD986F130.052.77160.620.50.4820.0181.011.28UMemphis
25R1523H3BXD957M730.143.978.360.4350.5470.0181.360.77UTM RW
26R1531H1BXD1156F630.062.22956.360.5050.4750.022.231.02Glenn
27R1367H1BXD1156M130.012.1178.780.5030.4770.021.071.27Glenn
28R1530H1BXD1258F1303.22753.770.5050.4770.0180.951.4Glenn
29R2674H1BXD1259M730.031.92483.440.5190.4640.0181.210.78Glenn
30R1529H1BXD1358F630.052.5559.050.4970.4850.01821.54Glenn
31R1662H2BXD1360M130.034.60345.810.5090.4720.0191.30.82Glenn
32R1304H2BXD1472F730.033.94661.870.4840.4980.0181.220.77UTM RW
33R1278H2BXD1455M730.064.7567.520.4490.5320.0191.10.73UTM RW
34R1524H1BXD1560F640.022.96150.930.4970.4840.0191.740.91Glenn
35R1515H1BXD1561M130.013.31657.050.5030.4780.0191.321.21Glenn
36R1661H1BXD1661F130.012.77859.810.5160.4660.0191.391.2Glenn
37R1594H1BXD1661M430.032.63453.660.5040.4780.0181.961.51Glenn
38R2666H1BXD1960F730.022.49876.20.4950.4860.0191.410.77Glenn
39R1471H1BXD19157M130.023.16543.340.5190.4620.0181.011.29UTM JB
40R1573H1BXD2059F130.023.74952.70.5130.4690.0181.011.27Glenn
41R2507H1BXD2060M630.063.568570.4720.5080.021.290.76Glenn
42R1347H2BXD2164F140.012.88161.490.4940.4860.0190.921.22UMemphis
43R2668H1BXD2160M740.072.60544.90.5350.4490.0171.540.76Glenn
44R1337H2BXD21102F2402.67358.050.4920.4890.0191.40.76UAB
45R1848H3BXD22196F640.022.94351.70.4940.4850.0212.20.78UAB
46R1525H1BXD2259M230.022.24855.760.5480.4330.0181.260.74Glenn
47R1280H2BXD2356F130.013.18754.630.4580.5230.0190.961.2UTM RW
48R1537H1BXD2358F530.13.71967.540.4680.5130.0191.510.96Glenn
49R1244H2BXD2365M730.051.25781.930.5650.4170.0181.240.74Glenn
50R1343H2BXD2471F230.012.08365.070.5060.4740.0191.460.75UMemphis
51R1517H1BXD2457M330.013.47153.660.5040.4760.0191.280.78Glenn
52R1366H1BXD2760F2402.2648.460.5180.4630.0191.290.77Glenn
53R1849H1BXD2770M530.068.80138.340.4680.5120.0192.421.08UAB
54R1353H1BXD2879F340.013.2276.220.480.50.021.330.78UMemphis
55R2332H1BXD2860M230.013.21763.680.4910.490.0191.370.79Glenn
56R1532H1BXD2957F230.012.12259.180.5240.4560.0191.170.76Glenn
57R1356H1BXD2976M530.014.03347.670.520.4630.0171.170.78UMemphis
58R1240H2BXD3161M230.022.33565.170.5070.4740.0191.310.78UTM RW
59R1526H2BXD3157F740.17.26789.540.4350.5470.0171.350.78UTM RW
60R2675H1BXD3257F730.032.26878.010.5020.4780.021.220.78Glenn
61R1508H2BXD3258M240.011.91767.780.5390.4420.0191.280.73Glenn
62R1345H3BXD3365F220.012.09863.140.5220.4590.0191.270.73UMemphis
63R1581H1BXD3359M330.013.22953.160.4960.4850.0191.190.78Glenn
64R1527H1BXD3459F230.012.358.920.510.4710.0191.240.76Glenn
65R1339H3BXD3474M530.122.88853.490.5060.4760.0182.391.35UMemphis
66R1469H1BXD3683F330.023.47349.90.4940.4860.021.110.76UMemphis
67R1363H1BXD3677M240.012.18448.190.5380.4430.021.280.77UMemphis
68R1855H1BXD3855F340.013.53654.540.490.4920.0181.390.75Glenn
69R1510H1BXD3859M230.012.18668.060.5210.460.0191.260.79Glenn
70R1528H2BXD3959F230.034.71738.30.5110.470.021.120.75Glenn
71R1514H1BXD3959M330.033.99256.060.4770.5040.0191.430.81Glenn
72R1522H1BXD4059F4402.63167.160.490.4910.0181.560.77Glenn
73R1359H1BXD4073M230.097.45839.860.4510.5270.0211.280.74UMemphis
74R1541H2BXD4258F730.076.78452.120.4830.4990.0171.130.66Glenn
75R1540H1BXD4258M740.032.42375.140.4920.4880.021.480.78Glenn
76R1334H2BXD4359F1302.67254.360.4920.4910.0171.22.06UTM RW
77R1303H1BXD4363M340.023.49751.90.4860.4950.0191.150.8UTM RW
78R1326H1BXD4465F3403.41253.960.4960.4850.0181.350.78UTM RW
79R1577H2BXD4456M130.022.15967.520.5120.4690.0191.181.71UTM RW
80R1403H2BXD4563F720.033.14644.50.5240.4570.0181.410.78Glenn
81R1472H1BXD4565M740.041.65173.310.5430.440.0181.630.74UTM RW
82R1316H1BXD4858F4302.44568.590.5150.4670.0191.160.73UTM RW
83R1575H3BXD4865M340.054.57755.780.4660.5140.0191.590.9UTM RW
84R2521H1BXD5063F640.013.10957.280.4950.4850.021.230.78UTM RW
85R1944H2BXD5081M130.012.54663.390.4950.4850.020.91.57UTM RW
86R2331H1BXD5166F330.033.53444.420.5010.4810.0171.20.9UTM RW
87R1582H1BXD5171M640.032.9247.870.4890.4910.021.360.75UTM RW
88R2680H1BXD5565M730.071.70779.750.5030.480.0171.911.05UTM RW
89R1331H1BXD6060F430.012.86750.330.4920.4870.0211.340.78UTM RW
90R1281H2BXD6059M1302.3958.440.5110.4690.020.941.2UTM RW
91R2667H1BXD6170F740.033.3659.040.4950.4880.0181.160.76UTM RW
92R1856H2BXD6194M1203.50249.60.5010.480.0190.961.3UTM RW
93R1246H1BXD6254F140.023.40551.470.5110.4710.0181.141.34UTM RW
94R1585H2BXD6264M640.013.15655.770.5180.4640.0181.430.82UTM RW
95R1945H1BXD63107F130.022.81152.650.5220.4590.0191.051.36UTM RW
96R2093H3BXD6370M630.023.89442.850.5030.4770.0191.291.01UTM RW
97R2062H2BXD6465F130.053.79578.480.5130.4680.0190.981.43UTM RW
98R2061H1BXD6487M340.013.53661.570.4770.5040.0191.310.78UTM RW
99R2054H2BXD6555F120.033.15980.960.480.5020.0181.091.24UTM RW
100R2056H2BXD6589M6202.83659.60.5040.4770.0191.30.75UTM RW
101R1941H2BXD6678F140.012.73450.930.4990.4810.021.181.29UTM RW
102R1949H2BXD6696M420.042.82851.270.4740.5080.0192.051.12UTM RW
103R2060H1BXD6754F630.012.56143.880.5020.4790.021.70.84UTM RW
104R2052H1BXD6761M140.013.16143.230.5210.460.0181.091.31UTM RW
105R2074H1BXD6860F530.026.52849.620.4790.5020.0191.480.83UTM RW
106R1928H1BXD6872M220.012.40448.280.5210.4590.021.30.74UTM RW
107R1439H3BXD6960F230.022.46359.140.5220.4590.0181.310.78UTM RW
108R1559H1BXD6964M330.032.98767.740.4860.4960.0171.380.8UTM RW
109R2134H1BXD7064F520.022.14858.640.5320.450.0191.40.85UTM RW
110R2063H1BXD7055M230.023.48155.320.5130.4690.0181.280.71UTM RW
111R1277H1BXD7360F420.012.57662.450.5020.4790.0191.350.79UTM RW
112R1443H2BXD7376M230.012.31264.340.4990.4810.021.480.77UTM RW
113R2055H2BXD7479M230.012.57656.840.5090.4730.0181.460.88UTM RW
114R2316H1BXD74193M520.013.45755.350.5080.4710.021.170.78UTM RW
115R1871H1BXD7561F230.041.72356.40.530.4510.0191.30.76UTM RW
116R1844H2BXD7590M340.011.93456.230.520.4610.0191.620.86UTM RW
117R1948H2BXD7681F230.011.50768.850.5530.4280.021.30.75UTM RW
118R2094H1BXD7661M540.013.29942.690.5190.4620.0191.390.88UTM RW
119R2262H1BXD7762F340.024.31747.160.4930.4880.0191.320.74UTM RW
120R1423H1BXD7762M230.023.07154.150.510.4710.0191.260.74UTM RW
121R1947H1BXD79108F220.012.59951.520.5240.4570.0191.350.74UTM RW
122R2092H1BXD7986M540.063.73542.250.5140.4680.0182.941.06UTM RW
123R1880H1BXD8068F530.064.85542.220.5010.4810.0182.171.36UTM RW
124R1881H2BXD8068M230.022.07348.930.5240.4580.0191.340.83UTM RW
125R2075H1BXD8360F230.012.45455.10.5020.480.0181.270.77UTM RW
126R2076H2BXD8360M630.032.62455.650.4950.4880.0182.210.94UTM RW
127R2077H2BXD8462F6202.171.870.5220.4590.0181.680.81UTM RW
128R2135H3BXD8475M220.012.46764.460.5050.4760.0191.20.74UTM RW
129R1473H1BXD8579F230.023.38455.340.4780.5020.021.240.77UTM RW
130R1474H1BXD8557M130.012.83155.240.5220.4610.0181.041.29UTM RW
131R1597H1BXD8586M440.092.02853.950.4870.4920.0211.280.83UTM RW
132R1415H1BXD8677F430.022.52553.160.4950.4850.021.660.91UTM RW
133R2669H2BXD8763F730.072.6157.590.5130.470.0181.60.91UTM RW
134R1710H1BXD8784M240.012.69756.40.5120.4690.0191.280.79UTM RW
135R1872H2BXD8990F220.023.01363.530.4920.4880.0211.220.72UTM RW
136R1850H3BXD8982M440.032.73644.890.4980.4830.0191.50.83UTM RW
137R2058H1BXD9061F230.013.38948.050.5020.4780.021.530.76UTM RW
138R1600H2BXD9074M740.033.26151.310.5170.4650.0181.160.75Glenn
139R1301H2BXD9258F230.023.54341.970.5220.460.0181.50.79UTM RW
140R1309H1BXD9259M430.051.65566.340.4980.4810.0211.520.82UTM RW
141R2057H1BXD9392F530.024.03344.410.5090.4710.021.220.78UTM RW
142R2059H1BXD9358M1303.05860.290.4930.4880.0191.181.37UTM RW
143R2313H1BXD9459F3303.09159.450.4870.4950.0181.340.73UTM RW
144R1915H1BXD9665F520.045.14546.190.5020.4810.0171.370.74UTM RW
145R1846H2BXD9663M1303.15955.850.4870.4930.020.921.26UTM RW
146R2648H1BXD9774F740.021.66482.080.5180.4640.0191.40.78UTM RW
147R1927H2BXD9767M130.042.62257.810.5390.4440.0171.451.32UTM RW
148R1942H1BXD9862F530.043.10448.420.5280.4540.0192.221.08UTM RW
149R1943H2BXD9862M330.024.0456.850.4840.4970.0191.180.76UTM RW
150R2197H1BXD9970F330.024.28851.750.490.4920.0181.350.81UTM RW
151R2315H1BXD9984M520.036.03643.050.4840.4970.0181.70.96UTM RW
152R2038H3C3H/HeJ63F630.022.67166.740.4760.5040.021.410.77UTM RW
153R2039H1C3H/HeJ63M530.13.38444.150.5280.4540.0172.160.88UTM RW
154R2137H1C57BL/6ByJ55F530.024.74647.010.4880.4930.0181.230.79JAX
155R2673H1C57BL/6ByJ55M730.081.84267.690.5140.4690.0171.750.78JAX
156R1361H1C57BL/6J69F640.013.05851.870.4770.5030.021.670.76UTM RW
157R2041H2C57BL/6J65M140.043.34149.260.5270.4560.0181.141.45UTM RW
158R1449H2C57BL/6J71M530.093.59244.320.470.510.021.680.77UTM DG
159R2619H1CAST/Ei64F530.144.07751.870.4550.5280.0182.741.2JAX
160R2116H1CXB155F330.075.79251.590.4590.5210.021.170.8JAX
161R2096H1CXB155M420.013.43553.780.4950.4850.021.220.79JAX
162R2124H1CXB1053F420.114.86739.880.4510.5280.021.550.8JAX
163R2671H1CXB1053M730.092.34871.450.4880.4940.0182.21.14JAX
164R2125H1CXB1158F330.033.25654.950.4610.5190.021.460.77JAX
165R2128H1CXB1158M420.064.98654.130.4650.5150.021.110.83JAX
166R2126H1CXB1247F430.113.93554.110.4690.5110.0211.50.79JAX
167R2109H1CXB1247M330.074.51849.260.4880.4920.021.230.77JAX
168R2672H1CXB1349F730.031.72279.520.5160.4650.0191.640.75JAX
169R2110H1CXB1356M430.213.47848.080.4610.5170.0221.210.78JAX
170R2117H2CXB262F420.043.3945.970.5330.450.0172.050.89JAX
171R2098H1CXB268M330.022.57254.220.4960.4850.0191.380.86JAX
172R2118H1CXB347F330.033.64663.160.4780.5030.0191.220.77JAX
173R2100H1CXB347M430.025.7651.380.480.5030.0171.240.81JAX
174R2119H1CXB458F430.023.89749.210.4880.4940.0181.310.79JAX
175R2101H1CXB458M330.137.37253.770.4330.5480.0191.20.97JAX
176R2505H1CXB580F630.022.8349.60.4990.480.021.330.76UTM RW
177R2131H1CXB542M430.15.57751.150.4340.5470.0191.70.89JAX
178R0129H2CXB570M330.074.82945.420.4880.4930.0191.230.83UTM RW
179R2676H1CXB647F720.052.14662.510.5070.4750.0181.520.78JAX
180R2102H1CXB649M430.075.14851.630.4530.5290.0181.430.87JAX
181R2121H1CXB763F420.064.90448.710.4640.5170.0191.190.92JAX
182R2104H2CXB758M320.063.38948.790.5020.4790.0191.741.48JAX
183R2122H1CXB854F330.044.12859.770.4510.5290.021.120.76JAX
184R2105H1CXB841M430.163.14661.040.4510.530.0191.340.84JAX
185R2123H1CXB954F330.085.70855.940.4380.5430.0191.320.78JAX
186R2106H1CXB954M430.065.86846.550.4690.5120.0191.180.82JAX
187R2045H2D2B6F165F120.014.40347.990.4970.4850.0181.091.53UTM RW
188R1595H2D2B6F163F530.062.57958.490.5060.4750.0192.491.21UTM RW
189R1551H1D2B6F172F630.022.6253.760.5060.4760.0181.370.76UTM RW
190R1290H2DBA/2J63F720.042.57659.60.5130.4680.0181.30.78JAX
191R1468H1DBA/2J64F530.032.92953.80.5150.4650.0191.280.79UTM RW
192R1683H1KK/HIJ72F630.023.91954.230.4910.4890.021.310.83JAX
193R1687H3KK/HIJ72M530.043.88840.860.4990.4830.0191.860.88JAX
194R2046H1LG/J63F520.032.82259.180.5140.4680.0181.680.8UTM RW
195R2047H2LG/J63M630.072.03860.340.5090.4710.022.160.95UTM RW
196R2048H1NOD/LtJ77F620.144.04550.210.4890.490.0212.890.95UTM RW
197R2049H3NOD/LtJ76M530.12.32852.780.5190.4620.0193.091.35UTM RW
198R2200H1NZO/HlLtJ62F520.032.64854.290.5430.4380.0191.270.8JAX
199R2350H1NZO/HlLtJ96M620.192.39150.520.5180.4630.023.712.21JAX
200R2677H1PWD/PhJ65F720.122.76465.490.4620.520.0181.891.16UTM RW
201R2051H3PWD/PhJ64M530.073.26651.50.4750.5060.0192.81.01UTM RW
202R2322H1PWK/PhJ63F520.092.9454.910.5110.470.0192.321.02JAX
203R2349H1PWK/PhJ83M620.153.30654.930.4590.5220.0194.651.45JAX
204R2198H2WSB/EiJ58F610.022.92257.970.5020.4790.0191.440.76JAX
205R2199H1WSB/EiJ58M530.043.17154.950.4750.5050.021.320.81JAX
+ +
+
+
+ +

    Downloading all data:

+
+

All data links (right-most column above) will be made active as sooon as the global analysis of these data by the Consoritum has been accepted for publication. Please see text on Data Sharing Policies, and Conditions and Limitations, and Contacts. Following publication, download a summary text file or Excel file of the PDNN probe set data. Contact RW Williams regarding data access probelms. + +

+
+ + + + +

    About the array platform:

+
+

Affymetrix Mouse Genome 430 2.0 array: The 430v2 array consists of 992936 useful 25-nucleotide probes that estimate the expression of approximately 16,578 NCBI Reference Sequences. The array sequences were selected late in 2002 using Unigene Build 107 by Affymetrix. The annotation used in this data set assigns probes to probe sets based on their alignment to Entrez GeneID sequences using the latest Mouse Genome assembly (Build 36, mm8).

+
+ +

    About data processing:

+ +
+Harshlight was used to examine the image quality of the array (CEL files). Bad areas (bubbles, scratches, blemishes) of arrays were masked. + +

First pass data quality control: Affymetrix GCOS provides useful array quality control data including: +

    +
  1. The scale factor used to normalize mean probe intensity. This averaged 3.3 for the 179 arrays that passed and 6.2 for arrays that were excluded. The scale factor is not a particular critical parameter. +
  2. The average background level. Values averaged 54.8 units for the data sets that passed and 55.8 for data sets that were excluded. This factor is not important for quality control. +
  3. The percentage of probe sets that are associated with good signal ("present" calls). This averaged 50% for the 179 data sets that passed and 42% for those that failed. Values for passing data sets extended from 43% to 55%. This is a particularly important criterion. +
  4. The 3':5' signal ratios of actin and Gapdh. Values for passing data sets averaged 1.5 for actin and 1.0 for Gapdh. Values for excluded data sets averaged 12.9 for actin and 9.6 for Gapdh. This is a highly discriminative QC criterion, although one must keep in mind that only two transcripts are being tested. Sequence variation among strains (particularly wild derivative strains such as CAST/Ei) may affect these ratios. +
+ +

The second step in our post-processing QC involves a count of the number of probe sets in each array that are more than 2 standard deviations (z score units) from the mean across the entire 206 array data sets. This was the most important criterion used to eliminate "bad" data sets. All 206 arrays were processed togther using standard RMA and PDNN methods. The count and percentage of probe sets in each array that were beyond the 2 z theshold was computed. Using the RMA transform the average percentage of probe sets beyond the 2 z threshold for the 179 arrays that finally passed of QC procedure was 1.76% (median of 1.18%). In contrast the 2 z percentage was more than 10-fold higher (mean of 22.4% and median 20.2%) for those arrays that were excluded. This method is not very senstive to the transformation method that is used. Using the PDNN transform the average percent of probe sets exceeding was 1.31% for good arrays and was 22.6% for those that were excluded. In our opinion, this 2 z criterion is the most useful criterion for the final decision of whether or not to include arrays, although again, allowances need to be made for wild strains that one expects to be different from the majority of conventional inbred strains. For examploe, if a data set has excellent characteristics on all of the Affymetrix GCOS metrics listed above, but generates a high 2 z percentage, then one whould include the ssample if one can verify that there are no problems in sample and data set identification. + +

The entire procedure can be reapplied once the initial outlier data sets have been eliminated to detect any remaining outlier data sets. + + + +

DataDesk was used to examine the statistical quality of the of the probe level (CEL) data after step 5 below. DataDesk allows a rapid detection of subsets of probes that are particular sensitive to still unknown factors in array processing. Arrays can then be categorized at the probe level into "reaction classes." A reaction class is a group of arrays for which the expression of essentially all probes are colinear over the full range of log2 values. A single but large group of arrays (n = 32) processed in essentially the identical manner by a single operator can produce arrays belonging to as many as four different reaction classes. Reaction classes are NOT related to strain, age, sex, treatment, or any known biological parameter (technical replicates can belong to different reaction classes). We do not yet understand the technical origins of reaction classes. The number of probes that contribute to the definition of reaction classes is quite small (<10% of all probes). We have categorized all arrays in this data set into one of 5 reaction classes. These have then been treated as if they were separate batches. Probes in these data type "batches" have been aligned to a common mean as described below. + + +

Probe set data with custom CDF mapping: The original Affymetrix annotation often has multiple probe sets mapping to a single gene. Some of these redundancies represent alternative splicing products, while some reflect our changing knowledge of the mouse genome. This transformation uses an annotation generated by the Microarray Group at the University of Michigan where each probe has been checked against the latest mouse genome build (Build 36, mm8) and then collated into a new probe set based on its placement within a gene sequence in the Entrez Gene database. The following quote from their Brainarray website explains in more detail: + +

+Affymetrix GeneChips were based on the best UniGene clustering and genomic sequence information available at the time of chip design. Due to the significant increase in EST/cDNA/Genomic sequence information in the last couple of years, some oligonucleotide probes in these old designs can now be assigned to different genes/transcripts based on the current UniGene clustering and genome annotation. While Affymetrix's current annotation system maps each probe set to the latest UniGene build every couple of months, it does not deal with situations where a subset of oligonucleotide probes in a probe set may be assigned to another gene or more than one gene based on the current UniGene clustering and genome annotation. +In addition, a significant portion of UniGene clusters can be represented by more than one oligonucleotide probe set on GeneChips but there is no standard approach to deal with signals from different probe sets representing the same gene. It will be highly desirable to have one probe set-one target relationship for the interpretation of the data. + + +

    + +
  1. CEL values produced by GCOS are 75% quantiles from a set of 91 pixel values per cell. + +
  2. Probe level data from the CEL files were transformed with the RMA transform using the Mm74Bv2_Mm_ENTREZG_8 (Version 8) CDF mapping. Data transformation was done in Bioconductor using the affy.justRMA() package and the Mm430_Mm_ENTREZG file as contained in the Bioconductor repository. This yields only one unique probeset for each Entrez GeneID. + +
  3. We computed the Z scores for each array. + +
  4. The arithmetic mean of the values for the set of microarrays for each strain was computed. + +
  5. The Z scores were recomputed for each strain. + +
  6. We multiplied all Z scores by 2. + +
  7. We added 8 to the value of all Z scores. The consequence of this simple set of transformations is to produce a set of Z scores that have a mean of 8, a variance of 4, and a standard deviation of 2. The advantage of this modified Z score is that a two-fold difference in expression level (probe brightness level) corresponds approximately to a 1 unit difference. + +
+ + +

Probe level QC: Log2 probe data of all arrays were inspected in DataDesk before and after quantile normalization. Inspection involved examining scatterplots of pairs of arrays for signal homogeneity (i.e., high correlation and linearity of the bivariate plots) and looking at all pairs of correlation coefficients. XY plots of probe expression and signal variance were also examined. Probe level array data sets were organized into reaction groups. Arrays with probe data that were not homogeneous when compared to other arrays were flagged. + +

Probe set level QC: The final normalized individual array data were evaluated for outliers. This involved counting the number of times that the probe set value for a particular array was beyond two standard deviations of the mean. This outlier analysis was carried out using the PDNN, RMA and MAS5 transforms and outliers across different levels of expression. Arrays that were associated with an average of more than 8% outlier probe sets across all transforms and at all expression levels were eliminated. In contrast, most other arrays generated fewer than 5% outliers. + + +

Validation of strains and sex of each array data set: A subset of probes and probe sets with a Mendelian pattern of inheritance were used to construct a expression correlation matrix for all arrays and the ideal Mendelian expectation for each strain constructed from the genotypes. There should naturally be a very high correlation in the expression patterns of transcripts with Mendelian phenotypes within each strain, as well as with the genotype strain distribution pattern of markers for the strain. + +

Sex of the samples was validated using sex-specific probe sets such as Xist and Dby. + + +

+ + +

    Data source acknowledgment:

+

Data were generated with funds provided by a variety of public and private source to members of the Consortium. All of us thank Muriel Davisson, Cathy Lutz, and colleagues at the Jackson Laboratory for making it possible for us to add all of the CXB strains, and one or more samples from KK/HIJ, WSB/Ei, NZO/HILtJ, LG/J, CAST/Ei, PWD/PhJ, and PWK/PhJ to this study. We thank Yan Cui at UTHSC for allowing us to use his Linux cluster to align all M430 2.0 probes and probe sets to the mouse genome. We thank Hui-Chen Hsu and John Mountz for providing us BXD tissue samples, as well as many strains of BXD stock. We thanks Douglas Matthews (UMem in Table 1) and John Boughter (JBo in Table 1) for sharing BXD stock with us. Members of the Hippocampus Consortium thank the following sources for financial support of this effort: + +

    +
  • David C. Airey, Ph.D. +
    Grant Support: Vanderbilt Institute for Integrative Genomics +
    Department of Pharmacology +
    david.airey at vanderbilt.edu + +
  • Lu Lu, M.D. +
    Grant Support: NIH U01AA13499, U24AA13513 + +
  • Fred H. Gage, Ph.D. + +
    Grant Support: Lookout Foundation + +
  • Dan Goldowitz, Ph.D. +
    Grant Support: NIAAA INIA AA013503 +
    University of Tennessee Health Science Center +
    Dept. Anatomy and Neurobiology +
    email: dgold@nb.utmem.edu + +
  • Shirlean Goodwin, Ph.D. +
    Grant Support: NIAAA INIA U01AA013515 + +
  • Gerd Kempermann, M.D. +
    Grant Support: The Volkswagen Foundation Grant on Permissive and Persistent Factors in Neurogenesis in the Adult Central Nervous System + +
    Humboldt-Universitat Berlin +
    Universitatsklinikum Charite +
    email: gerd.kempermann at mdc-berlin.de + +
  • Kenneth F. Manly, Ph.D. +
    Grant Support: NIH P20MH062009 and U01CA105417 + +
  • Richard S. Nowakowski, Ph.D. +
    Grant Support: R01 NS049445-01 + +
  • Yanhua Qu, Ph.D. +
    Grant Support: NIH U01CA105417 + +
  • Glenn D. Rosen, Ph.D. +
    Grant Support: NIH P20 + +
  • Leonard C. Schalkwyk, Ph.D. + +
    Grant Support: MRC Career Establishment Grant G0000170 +
    Social, Genetic and Developmental Psychiatry +
    Institute of Psychiatry,Kings College London +
    PO82, De Crespigny Park London SE5 8AF +
    L.Schalkwyk@iop.kcl.ac.uk + +
  • Guus Smit, Ph.D. +
    Dutch NeuroBsik Mouse Phenomics Consortium +
    Center for Neurogenomics & Cognitive Research +
    Vrije Universiteit Amsterdam, The Netherlands +
    e-mail: guus.smit at falw.vu.nl +
    Grant Support: BSIK 03053 + +
  • Thomas Sutter, Ph.D. +
    Grant Support: INIA U01 AA13515 and the W. Harry Feinstone Center for Genome Research + +
  • Stephen Whatley, Ph.D. + +
    Grant Support: XXXX + +
  • Robert W. Williams, Ph.D. +
    Grant Support: NIH U01AA013499, P20MH062009, U01AA013499, U01AA013513 + +
+ + + +

+ +

    About this text file:

+

+This text file originally generated by RWW and Rupert Overall on January 30, 2007. +

+ + +

+ +
+ + + + + + +
+ + + + +
+ + + + + + + + + + + -- cgit v1.2.3