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        Download the raw data used to create the plots in this report below:

        Note that additional data was saved in multiqc_data when this report was generated.


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        If you use plots from MultiQC in a publication or presentation, please cite:

        MultiQC: Summarize analysis results for multiple tools and samples in a single report
        Philip Ewels, Måns Magnusson, Sverker Lundin and Max Käller
        Bioinformatics (2016)
        doi: 10.1093/bioinformatics/btw354
        PMID: 27312411

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        Tool Citations

        Please remember to cite the tools that you use in your analysis.

        To help with this, you can download publication details of the tools mentioned in this report:

        About MultiQC

        This report was generated using MultiQC, version 1.12

        You can see a YouTube video describing how to use MultiQC reports here: https://youtu.be/qPbIlO_KWN0

        For more information about MultiQC, including other videos and extensive documentation, please visit http://multiqc.info

        You can report bugs, suggest improvements and find the source code for MultiQC on GitHub: https://github.com/ewels/MultiQC

        MultiQC is published in Bioinformatics:

        MultiQC: Summarize analysis results for multiple tools and samples in a single report
        Philip Ewels, Måns Magnusson, Sverker Lundin and Max Käller
        Bioinformatics (2016)
        doi: 10.1093/bioinformatics/btw354
        PMID: 27312411

        A modular tool to aggregate results from bioinformatics analyses across many samples into a single report.

        Report generated on 2022-08-09, 13:09 based on data in: /home/shared/8TB_HDD_02/mattgeorgephd/PSMFC-mytilus-byssus-pilot/fastqc/trimmed


        General Statistics

        Showing 73/73 rows and 3/5 columns.
        Sample Name% Dups% GCM Seqs
        T001FX_S219_R1
        64.0%
        38%
        4.6
        T001F_S100_R1
        65.8%
        38%
        5.1
        T001G_S112_R1
        43.1%
        36%
        5.0
        T002FX_S220_R1
        56.4%
        37%
        4.0
        T002F_S101_R1
        58.6%
        38%
        5.0
        T002G_S113_R1
        40.5%
        36%
        3.9
        T003FX_S221_R1
        57.0%
        37%
        4.6
        T003F_S102_R1
        65.6%
        40%
        4.8
        T003G_S114_R1
        40.9%
        35%
        4.4
        T004FX_S222_R1
        60.1%
        37%
        5.5
        T004F_S103_R1
        65.4%
        39%
        4.6
        T004G_S115_R1
        38.2%
        35%
        3.8
        T005FX_S223_R1
        59.7%
        37%
        4.8
        T005F_S104_R1
        64.7%
        38%
        3.9
        T005G_S116_R1
        40.0%
        35%
        5.5
        T006FX_S224_R1
        57.8%
        37%
        4.8
        T006F_S105_R1
        62.4%
        39%
        4.2
        T006G_S117_R1
        36.8%
        35%
        5.1
        T007FX_S225_R1
        63.0%
        39%
        4.2
        T007F_S106_R1
        68.4%
        38%
        5.3
        T007G_S118_R1
        38.6%
        36%
        4.0
        T008FX_S226_R1
        60.2%
        37%
        3.6
        T008F_S107_R1
        65.6%
        38%
        5.8
        T008G_S119_R1
        42.1%
        35%
        6.3
        T009FX_S227_R1
        58.8%
        37%
        4.4
        T009F_S108_R1
        59.0%
        38%
        4.4
        T009G_S120_R1
        40.1%
        35%
        5.3
        T010FX_S228_R1
        58.0%
        37%
        4.0
        T010F_S109_R1
        62.8%
        39%
        5.2
        T010G_S121_R1
        39.9%
        35%
        4.5
        T011FX_S229_R1
        57.0%
        37%
        4.0
        T011F_S110_R1
        59.0%
        37%
        3.7
        T011G_S122_R1
        38.4%
        35%
        4.6
        T012FX_S230_R1
        56.8%
        37%
        4.7
        T012F_S111_R1
        60.5%
        37%
        5.5
        T012G_S123_R1
        40.8%
        35%
        4.1
        T014F_S171_R1
        57.3%
        38%
        4.3
        T014G_S183_R1
        39.4%
        35%
        4.8
        T015F_S172_R1
        57.4%
        37%
        5.2
        T015G_S184_R1
        39.0%
        35%
        4.9
        T016F_S173_R1
        56.6%
        36%
        4.0
        T016G_S185_R1
        37.0%
        35%
        4.2
        T017F_S174_R1
        48.7%
        36%
        4.0
        T017G_S186_R1
        38.8%
        35%
        4.2
        T019F_S175_R1
        53.9%
        36%
        4.9
        T019G_S187_R1
        40.8%
        35%
        4.4
        T021F_S176_R1
        43.8%
        35%
        4.4
        T021G_S188_R1
        35.6%
        34%
        4.6
        T023F_S177_R1
        53.3%
        36%
        5.1
        T023G_S189_R1
        38.7%
        35%
        4.4
        T025F_S178_R1
        49.2%
        36%
        4.4
        T025G_S190_R1
        43.2%
        36%
        4.4
        T026F_S179_R1
        55.8%
        37%
        4.7
        T026G_S191_R1
        39.6%
        35%
        5.1
        T027F_S180_R1
        53.9%
        36%
        4.8
        T027G_S192_R1
        36.6%
        35%
        3.7
        T029F_S195_R1
        55.3%
        37%
        4.8
        T029G_S207_R1
        36.1%
        35%
        4.6
        T030F_S196_R1
        53.2%
        36%
        4.6
        T030G_S208_R1
        32.9%
        35%
        2.5
        T131G_S141_R1
        38.6%
        35%
        5.8
        T132F_S130_R1
        58.2%
        37%
        4.4
        T132G_S142_R1
        37.6%
        35%
        3.8
        T133F_S131_R1
        49.6%
        36%
        3.8
        T133G_S143_R1
        42.8%
        36%
        5.9
        T134F_S132_R1
        57.8%
        36%
        5.5
        T134G_S144_R1
        37.3%
        35%
        5.2
        T135F_S133_R1
        52.4%
        36%
        5.5
        T135G_S145_R1
        41.4%
        35%
        4.4
        T136F_S134_R1
        51.4%
        36%
        5.0
        T136G_S146_R1
        42.3%
        35%
        4.3
        T137F_S135_R1
        55.7%
        37%
        4.9
        T137G_S147_R1
        34.1%
        35%
        4.9

        FastQC

        FastQC is a quality control tool for high throughput sequence data, written by Simon Andrews at the Babraham Institute in Cambridge.

        Sequence Counts

        Sequence counts for each sample. Duplicate read counts are an estimate only.

        This plot show the total number of reads, broken down into unique and duplicate if possible (only more recent versions of FastQC give duplicate info).

        You can read more about duplicate calculation in the FastQC documentation. A small part has been copied here for convenience:

        Only sequences which first appear in the first 100,000 sequences in each file are analysed. This should be enough to get a good impression for the duplication levels in the whole file. Each sequence is tracked to the end of the file to give a representative count of the overall duplication level.

        The duplication detection requires an exact sequence match over the whole length of the sequence. Any reads over 75bp in length are truncated to 50bp for this analysis.

        loading..

        Sequence Quality Histograms

        The mean quality value across each base position in the read.

        To enable multiple samples to be plotted on the same graph, only the mean quality scores are plotted (unlike the box plots seen in FastQC reports).

        Taken from the FastQC help:

        The y-axis on the graph shows the quality scores. The higher the score, the better the base call. The background of the graph divides the y axis into very good quality calls (green), calls of reasonable quality (orange), and calls of poor quality (red). The quality of calls on most platforms will degrade as the run progresses, so it is common to see base calls falling into the orange area towards the end of a read.

        loading..

        Per Sequence Quality Scores

        The number of reads with average quality scores. Shows if a subset of reads has poor quality.

        From the FastQC help:

        The per sequence quality score report allows you to see if a subset of your sequences have universally low quality values. It is often the case that a subset of sequences will have universally poor quality, however these should represent only a small percentage of the total sequences.

        loading..

        Per Base Sequence Content

        The proportion of each base position for which each of the four normal DNA bases has been called.

        To enable multiple samples to be shown in a single plot, the base composition data is shown as a heatmap. The colours represent the balance between the four bases: an even distribution should give an even muddy brown colour. Hover over the plot to see the percentage of the four bases under the cursor.

        To see the data as a line plot, as in the original FastQC graph, click on a sample track.

        From the FastQC help:

        Per Base Sequence Content plots out the proportion of each base position in a file for which each of the four normal DNA bases has been called.

        In a random library you would expect that there would be little to no difference between the different bases of a sequence run, so the lines in this plot should run parallel with each other. The relative amount of each base should reflect the overall amount of these bases in your genome, but in any case they should not be hugely imbalanced from each other.

        It's worth noting that some types of library will always produce biased sequence composition, normally at the start of the read. Libraries produced by priming using random hexamers (including nearly all RNA-Seq libraries) and those which were fragmented using transposases inherit an intrinsic bias in the positions at which reads start. This bias does not concern an absolute sequence, but instead provides enrichement of a number of different K-mers at the 5' end of the reads. Whilst this is a true technical bias, it isn't something which can be corrected by trimming and in most cases doesn't seem to adversely affect the downstream analysis.

        Click a sample row to see a line plot for that dataset.
        Rollover for sample name
        Position: -
        %T: -
        %C: -
        %A: -
        %G: -

        Per Sequence GC Content

        The average GC content of reads. Normal random library typically have a roughly normal distribution of GC content.

        From the FastQC help:

        This module measures the GC content across the whole length of each sequence in a file and compares it to a modelled normal distribution of GC content.

        In a normal random library you would expect to see a roughly normal distribution of GC content where the central peak corresponds to the overall GC content of the underlying genome. Since we don't know the the GC content of the genome the modal GC content is calculated from the observed data and used to build a reference distribution.

        An unusually shaped distribution could indicate a contaminated library or some other kinds of biased subset. A normal distribution which is shifted indicates some systematic bias which is independent of base position. If there is a systematic bias which creates a shifted normal distribution then this won't be flagged as an error by the module since it doesn't know what your genome's GC content should be.

        loading..

        Per Base N Content

        The percentage of base calls at each position for which an N was called.

        From the FastQC help:

        If a sequencer is unable to make a base call with sufficient confidence then it will normally substitute an N rather than a conventional base call. This graph shows the percentage of base calls at each position for which an N was called.

        It's not unusual to see a very low proportion of Ns appearing in a sequence, especially nearer the end of a sequence. However, if this proportion rises above a few percent it suggests that the analysis pipeline was unable to interpret the data well enough to make valid base calls.

        loading..

        Sequence Length Distribution

        The distribution of fragment sizes (read lengths) found. See the FastQC help

        loading..

        Sequence Duplication Levels

        The relative level of duplication found for every sequence.

        From the FastQC Help:

        In a diverse library most sequences will occur only once in the final set. A low level of duplication may indicate a very high level of coverage of the target sequence, but a high level of duplication is more likely to indicate some kind of enrichment bias (eg PCR over amplification). This graph shows the degree of duplication for every sequence in a library: the relative number of sequences with different degrees of duplication.

        Only sequences which first appear in the first 100,000 sequences in each file are analysed. This should be enough to get a good impression for the duplication levels in the whole file. Each sequence is tracked to the end of the file to give a representative count of the overall duplication level.

        The duplication detection requires an exact sequence match over the whole length of the sequence. Any reads over 75bp in length are truncated to 50bp for this analysis.

        In a properly diverse library most sequences should fall into the far left of the plot in both the red and blue lines. A general level of enrichment, indicating broad oversequencing in the library will tend to flatten the lines, lowering the low end and generally raising other categories. More specific enrichments of subsets, or the presence of low complexity contaminants will tend to produce spikes towards the right of the plot.

        loading..

        Overrepresented sequences

        The total amount of overrepresented sequences found in each library.

        FastQC calculates and lists overrepresented sequences in FastQ files. It would not be possible to show this for all samples in a MultiQC report, so instead this plot shows the number of sequences categorized as over represented.

        Sometimes, a single sequence may account for a large number of reads in a dataset. To show this, the bars are split into two: the first shows the overrepresented reads that come from the single most common sequence. The second shows the total count from all remaining overrepresented sequences.

        From the FastQC Help:

        A normal high-throughput library will contain a diverse set of sequences, with no individual sequence making up a tiny fraction of the whole. Finding that a single sequence is very overrepresented in the set either means that it is highly biologically significant, or indicates that the library is contaminated, or not as diverse as you expected.

        FastQC lists all of the sequences which make up more than 0.1% of the total. To conserve memory only sequences which appear in the first 100,000 sequences are tracked to the end of the file. It is therefore possible that a sequence which is overrepresented but doesn't appear at the start of the file for some reason could be missed by this module.

        loading..

        Adapter Content

        The cumulative percentage count of the proportion of your library which has seen each of the adapter sequences at each position.

        Note that only samples with ≥ 0.1% adapter contamination are shown.

        There may be several lines per sample, as one is shown for each adapter detected in the file.

        From the FastQC Help:

        The plot shows a cumulative percentage count of the proportion of your library which has seen each of the adapter sequences at each position. Once a sequence has been seen in a read it is counted as being present right through to the end of the read so the percentages you see will only increase as the read length goes on.

        loading..

        Status Checks

        Status for each FastQC section showing whether results seem entirely normal (green), slightly abnormal (orange) or very unusual (red).

        FastQC assigns a status for each section of the report. These give a quick evaluation of whether the results of the analysis seem entirely normal (green), slightly abnormal (orange) or very unusual (red).

        It is important to stress that although the analysis results appear to give a pass/fail result, these evaluations must be taken in the context of what you expect from your library. A 'normal' sample as far as FastQC is concerned is random and diverse. Some experiments may be expected to produce libraries which are biased in particular ways. You should treat the summary evaluations therefore as pointers to where you should concentrate your attention and understand why your library may not look random and diverse.

        Specific guidance on how to interpret the output of each module can be found in the relevant report section, or in the FastQC help.

        In this heatmap, we summarise all of these into a single heatmap for a quick overview. Note that not all FastQC sections have plots in MultiQC reports, but all status checks are shown in this heatmap.

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