Create a microarray design from HD CGH/ChIP database probes (Wizard)

The name of the control grid appears as a link. Click the link to view details about the control grid. eArray automatically selects a control grid appropriate to your design format, application type, and, for CGH and ChIP applications, species. If

appears in Control Grid, you can choose an alternate control grid.

A control grid is a set of control probes that are added to every array design. For every Agilent microarray design format and species there is a default species specific control grid suggested in eArray. These grids contain positive controls probes designs against endogenous sequence. Positive controls can be used for image orientation and to assess whether the sample was labeled. The “genomic” control grids are generic grids that contain only negative controls. Since they lack endogenous positive control probes they can be used for any species. The negative control probes are used to measure on element background. Here are some of the probe types you should expect to find on a species-specific genomic control grid.

BrightCorner (e.g., HsCGHBrightCorner)

Used for orientation purposes. These probes are placed in the corners of the array with a different pattern for each corner.
These probes are designed to endogenous sequence and are thus species-specific. These probes are predicted to have high signal due to the multiple copies found in the genome.

DarkCorner (DarkCorner)

Used for orientation purposes in the array corners. These, along with the bright corner probes, make up the corner-specific patterns.
These probes are the same as the 3xSLv1 probes described below.

Negative controls

Structural negative (3xSLv1)
- Usually highly replicated on the array; used to measure on element background. This probe forms a hairpin and does not hybridize well with labeled sample of any species.
Biological negatives (e.g., NC1_00000002)
- These are probes shown not to have significant signal from any sample tested. These probes are used to estimate on element background.
- Currently there are 82 different negative control NC probes.
- Common practice is to have one highly replicated NC probe (>100) and the other NC probes at lower replication (≈6).
Reserve negatives (e.g., SM_01)
- There are currently 12 sequences replicated 40 times marked as control type Positive that are reserved negative controls for future potential use as positive controls. They do not show significant signal from any sample tested.

Positive controls

Biological positives (e.g., RnPC_10045851, PC_00000004)
- Endogenous “species-specific” sequences predicted to have high signal, due to multiple copies found in the targeted genome, are used as positive controls. This is the same probe sequence used as the BrightCorner probe.
- Common practice is to have this probe highly replicated.
Deletion stringency probes (e.g., DCP_008001.0)
- Probes designed against endogenous “species-specific” sequence can be used to measure hybridization and wash stringency.
- Approximately 20 probes, predicted to perform well by in silico metrics, are chosen randomly from a tiling database and printed on the array in triplicate. In addition, four variants of this probe are printed on the array, also in triplicate. The first variant has a one base pair deletion, the second a three base pair deletion, and the third has a five base pair deletion, and finally the fourth variant has a seven base pair deletion. Bases to be deleted are chosen at random from the center of the probe sequence. The number of bases deleted is indicated by the number after the period. For example, DCP_008001.0 and DCP_008001.3 are from the same parent sequence and the first probe has zero deletions while the second has three.
Intensity curve probes (e.g., SRN_800001)
- Approximately two thousand species-specific probes are chosen to have predicted signals that span the practical signal space. These signal intensities are predictions made using an in-house model. These probes are generally not replicated.
- These probes can be used in a non-linear normalization.

Parameter	Instructions/Details
Probe Group Name	Type a name for the probe group. This name identifies the probe group in search results, lists of probe groups, and the like.
Status	Select Incomplete or Locked. If you select a status of Locked, you will not be able to further edit the probe group.
Description	(Optional) Type a brief description of the probe group.
Keywords	(Optional) Type keywords to associate with the probe group. Keywords can facilitate searches for the probe group. Separate multiple keywords with commas.
Folder	Select a location for the new probe group. The folders to which you have access appear in the list.

Parameter	Instructions/Details
Define Design
Microarray Name	Type a name for the microarray design. eArray uses this name as one of the search keys for microarray designs, and as a way to refer to the design in search results, lists, and the like.
Design Format	Select a design format. The design format defines the number of replicate arrays that each glass microarray slide contains, and the number and position of features in each array. For details about the selected design format, click Show Details. When you select or change the design format, an appropriate control grid appears in Control Grid.
Control Grid	The name of the control grid appears as a link. Click the link to view details about the control grid. eArray automatically selects a control grid appropriate to your design format, application type, and, for CGH and ChIP applications, species. If appears in Control Grid, you can choose an alternate control grid. To choose an alternate control grid: In Control Grid, click . A list of available control grids appears in a new window. Select the desired control grid, then click Done. What is a CGH control grid and which probes does it contain? A control grid is a set of control probes that are added to every array design. For every Agilent microarray design format and species there is a default species specific control grid suggested in eArray. These grids contain positive controls probes designs against endogenous sequence. Positive controls can be used for image orientation and to assess whether the sample was labeled. The “genomic” control grids are generic grids that contain only negative controls. Since they lack endogenous positive control probes they can be used for any species. The negative control probes are used to measure on element background. Here are some of the probe types you should expect to find on a species-specific genomic control grid. BrightCorner (e.g., HsCGHBrightCorner) Used for orientation purposes. These probes are placed in the corners of the array with a different pattern for each corner. These probes are designed to endogenous sequence and are thus species-specific. These probes are predicted to have high signal due to the multiple copies found in the genome. DarkCorner (DarkCorner) Used for orientation purposes in the array corners. These, along with the bright corner probes, make up the corner-specific patterns. These probes are the same as the 3xSLv1 probes described below. Negative controls Structural negative (3xSLv1) Usually highly replicated on the array; used to measure on element background. This probe forms a hairpin and does not hybridize well with labeled sample of any species. Biological negatives (e.g., NC1_00000002) These are probes shown not to have significant signal from any sample tested. These probes are used to estimate on element background. Currently there are 82 different negative control NC probes. Common practice is to have one highly replicated NC probe (>100) and the other NC probes at lower replication (≈6). Reserve negatives (e.g., SM_01) There are currently 12 sequences replicated 40 times marked as control type Positive that are reserved negative controls for future potential use as positive controls. They do not show significant signal from any sample tested. Positive controls Biological positives (e.g., RnPC_10045851, PC_00000004) Endogenous “species-specific” sequences predicted to have high signal, due to multiple copies found in the targeted genome, are used as positive controls. This is the same probe sequence used as the BrightCorner probe. Common practice is to have this probe highly replicated. Deletion stringency probes (e.g., DCP_008001.0) Probes designed against endogenous “species-specific” sequence can be used to measure hybridization and wash stringency. Approximately 20 probes, predicted to perform well by in silico metrics, are chosen randomly from a tiling database and printed on the array in triplicate. In addition, four variants of this probe are printed on the array, also in triplicate. The first variant has a one base pair deletion, the second a three base pair deletion, and the third has a five base pair deletion, and finally the fourth variant has a seven base pair deletion. Bases to be deleted are chosen at random from the center of the probe sequence. The number of bases deleted is indicated by the number after the period. For example, DCP_008001.0 and DCP_008001.3 are from the same parent sequence and the first probe has zero deletions while the second has three. Intensity curve probes (e.g., SRN_800001) Approximately two thousand species-specific probes are chosen to have predicted signals that span the practical signal space. These signal intensities are predictions made using an in-house model. These probes are generally not replicated. These probes can be used in a non-linear normalization.
Folder	Select a location for your new microarray design. The folders to which you have access appear in the list.
Description	(Optional) Type a brief description for the design.
Species	(Read-only) Reflects the species (if any) that you selected in the previous step of the wizard.
Keywords	(Optional) Type search keywords to associate with the design, separated by commas. Keywords can help you search for the microarray design later.
Attachment	(Optional) Attachments are files or links that are related your microarray design. Attached files should not exceed 32 Mb in size. To add one or more attachments, follow these steps: Click . A page appears in a new window. In the Attach pane, specify the following: Name – Type a name for the attachment. This name becomes the link you click to access the attachment. Type – Select the desired type of attachment from the list. An attachment can be either a file or a URL. Locale – Select the appropriate locale from the list. eArray uses this option to select content that has been localized for your region, when it is available. File – (Available only if you selected File for the type of attachment) Click Browse... Select the desired attachment in the dialog box that appears, then click Open. URL – (Available only if you selected URL for the type of attachment) Type the full URL of the Internet resource, including the protocol specifier. For example, http://www.agilent.com. Click Add. The attachment appears in the Attachment Header List at the top of the window. A success message appears. Click Close. Add additional attachments, if desired. If you add an attachment in error, select the check box next to its name in the Attachment Header List, then click Remove. Click Done. The window closes. The names of your attachments appear as links in Attachment.
Comments	(Optional) Type comments to include with the microarray design.
Linker Details
Append linker to 3' end	Mark this check box to add linker sequences to your probes. Linkers are nucleic acid molecules that are added to the 3' ends of probes. They move the "active" (hybridizing) sequence farther from the glass microarray substrate. This decreases steric hindrance and makes the sequence more available for hybridization. Linker sequences themselves are designed to avoid hybridization to any sequence in the target sample. Agilent provides a default linker sequence that you can use, or you can specify your own custom linker sequence. If you mark this option, also set the Linker Length and Linker Sequence parameters. For CGH microarrays, when should I choose to append linkers? For probes selected from the Agilent HD-CGH database, linkers are automatically added. For other probes, like probes generated through ‘Genomic Tiling’, Agilent recommends adding linkers in order to move the active probe sequences farther off of the array surface. This becomes more important for shorter sequences.
Linker length	(Available if you select Append linker to 3' end) Select one of these options: Make probes of length – Adds nucleotides to the 3' ends of probes so that the resulting probes (active sequence plus linker) have the length specified. Type a number of nucleotides from 20 and 60 in the box. If an active probe sequence in your microarray design exceeds the length that you specify, eArray leaves it alone. It is not trimmed, and no linker is appended to it. Add linker of length – Adds the specified number of nucleotides to the 3' ends of probes. Type a number of nucleotides from 1 to 49. With this option, eArray can produce probes of up to 60 nucleotides in length. If the active probe sequences have different lengths, the resultant probes will also have different lengths after linkers are appended. If the linker sequence is shorter than the length that you specify, eArray replicates the linker sequence to fill in the length.
Linker Sequence	(Available if you select Append linker to 3' end) Select one of these options: Use Agilent linker sequence – You cannot edit the sequence of the Agilent-provided linker. Use Customer linker sequence – Type a DNA base sequence for the linker. Provide a linker sequence that does not hybridize to any sequences in the target sample. Note: eArray appends the Agilent linker sequence to Agilent probes, even if you select Use Customer linker sequence.

Task	Instructions/Details
Add or remove a biological or user control probe group	You can add or remove a biological or user control probe group from your microarray design. To add a biological or user control probe group Click Biological <type> Probe Group Details, then click Add. A probe group selection page appears in a new window. Select one ore more probe groups as described in Select probe groups for probe searches. To add more probe groups, click Add again. Select the desired control type for each probe group. See below, Change control type of probe group. To remove a biological or user control probe group Click Biological <type> Probe Group Details, then mark the check box next to the probe group that you want to remove. Click Remove. Note: Separate tasks below describe how to add or remove normalization or replicate probe groups.
Add or remove a normalization probe group	(CGH arrays only) A normalization probe group is a special control probe group that provides data that can be used to normalize the two dye channel data generated from the array. When you create an array for certain species and design formats, eArray automatically adds a default Agilent normalization probe group. If normalization probe group(s) appear in your design, you can download a list of unique probes to use in the Agilent Feature Extraction (FE) program. The name of this file is Agilent dye normalization probe list for FE. To add a normalization probe group Click Normalization Probe Group Details, then click Add. A probe group selection page appears. Select one or more probe groups as described in Select probe groups for probe searches. The selected probe group(s) appear in Probe Group name. Note: When you add a normalization probe group to a microarray set, eArray places a copy of this probe group on every array within the set. To remove a normalization probe group Click Normalization Probe Group Details, then mark the check box next to the probe group that you want to remove. Click Remove.
Add or remove a replicate probe group	(CGH and Expression arrays only) A replicate probe group is a special control probe group that Feature Extraction and DNA Analytics can use to calculate the QC metric Reproducibility. These replicate probe groups are distinct from the user probe groups that you can include in designs in multiple copies. When you create an array for certain species and design formats, eArray automatically adds a default Agilent replicate probe group. To add a replicate probe group Click Replicate Probe Group Details, then click Add. A probe group selection page appears. Select one or more probe groups as described in Select probe groups for probe searches. The selected probe group(s) appear in Probe Group name. In Replicate, type the number of copies of the probe group to be included in the design. Agilent recommends a value of 5. Note: When you add a replicate probe group to a microarray set, eArray places the specified number of copies of this probe group on every array within the set. To remove a replicate probe group Click Replicate Probe Group Details, then mark the check box next to the probe group that you want to remove. Click Remove.
View a probe group	In any available Probe Group Name column, click the name of the probe group that you want to view. The View Probe Group page appears in a new window. For details about this page, see View probe group.
Change control type of probe group	(When available) Under Biological <type> Probe Group(s), next to the applicable probe group, in the Control Type column, select an option. Positive or negative user control probe groups must collectively occupy 50% or fewer of the available features in your design/set. neg – Designates the probe group as a negative user control. Negative control groups are intended to have no hybridization. The control grid that is assigned automatically to each design contains an adequate number of negative controls. If you assign your own additional group of negative controls, these negative controls are used by Feature Extraction for background determination (whether or not they have only background signal). pos – Designates the probe group as a positive user control. Although positive controls are excluded from many of the statistical QC metrics in Feature Extraction, they are available for downstream analysis. Positive controls generally have predictable signals, but this is not a requirement. An example of positive controls present on the Agilent control grid is the Agilent spike-in probes, which are used in the gene expression application for calculating QC metrics following addition of spike-in controls to the sample. ignore – Omits the probe group from Feature Extraction analyses and output. Once an array design is submitted, the Control Types cannot be changed, so the only way to "re-activate" them, if desired, is to modify the ControlType field of the design file. biological – Designates that the probe group is not a control (condition = FALSE). It is the default choice for biological probes, which should comprise at least 50% of your design. Note: In a microarray set, if you change the control type of a probe group to either neg or pos, you must also select a probe distribution option.
Change number of copies of probe group	(Available for non-control probe groups. For CGH and Expression designs, also available for replicate probe groups.) In the Replicate column, next to the desired probe group, type the number of copies of the probe group that you want to include in the microarray design.
Allow eArray to create a microarray set	Mark Enable Microarray Set. If you select this option, and the number of features required to accommodate your microarray design exceeds the number of features available on one microarray slide, eArray adds as many additional slides as are needed. The Percentage Filled statistic in the Microarray Statistics pane can help you to monitor how full your microarray is. If the percentage filled exceeds 100%, you must mark Enable Microarray Set to accommodate all the probes of your design, or choose a different design format with more feature locations. For positive or negative user control probe groups in a microarray set, you must also select a probe distribution option. Note: Once you create an individual microarray design, you cannot subsequently convert it into a microarray set, even if you add additional probes and exceed the capacity of the selected design format. Similarly, once you create a microarray set, you cannot convert it into an individual microarray design.
Change distribution of positive and negative control probe groups in a microarray set	(Available for microarray sets that have probe groups with a control type of pos or neg) eArray always puts a copy of each positive and negative user control probe group onto each microarray within a microarray set. Within each microarray in the set, the probes in the control probe groups are always assigned to random feature positions. However, you have some control over how probes are assigned to these randomly-selected feature positions from one array to another in the set. Click Biological <type> Probe Group(s). In the Control Probe Positioning column, select one of these options for each positive or negative user control probe group: Variable Random – Each positive or negative control probe appears on each microarray in the set in a different position. Example: eArray assigns Probe A randomly to feature position 4330 in one microarray in the set. In another microarray in the set, it might assign Probe A to feature position 961. Fixed Random – A given positive or negative control probe appears on each microarray in the set in the same position. Example: eArray assigns Probe A randomly to feature position 4330 in one microarray in the set. In all of the other microarrays in the set, Probe A is also assigned to feature position 4330. Note: For all other types of probe groups, eArray always assigns them to feature positions in a specific way: • Probe groups with a control type of biological or ignore – For each replicate requested, eArray distributes a single copy of the probe group randomly over all of the microarrays in the set. • Probe groups in the Replicate Probe Group Details pane or in the Normalization Probe Group Details pane – When these type(s) of probe groups are included in a microarray set, eArray places a copy of each one on every microarray in the set using Variable Random positioning. • Agilent quality control grid – With the exception of the SureSelect Capture Array application type, a set of these probes appears on every microarray in the set. The placement of these probes is the same on every array, and is defined by the control grid specifications.
Fill unused features	You can fill the unused features of a microarray with the probe group of your choice. eArray may add only part of the probe group or more than one copy of some or all of the probe group, depending on the number of available empty features in your design, and the number of probes in the probe group. To add a whole probe group to your design, use the procedure described above in Add a user control or non-control probe group, instead. Follow these steps to fill unused features: Mark Fill Microarrays. In Probe Group To Fill Microarray, click . A probe group selection page appears in a new window. For instructions on how to use this page, see Select probe groups for probe searches. Guidance from Agilent on unused CGH microarray features When designing a CGH microarray, if there are vacant, empty features after probes are selected, what does Agilent recommend as the next step? Should I increase the number of replicates or density? What are the pros and cons of increasing the number of replicates or increasing density? Blanks are not recommended, because Autogridding in Feature Extraction will become problematic. If the design you have selected does not fill the array, the following are Agilent recommended options, ordered by preference: 1. Choose a smaller array format. 2. Replicate all probes on the microarray. 3. Fill array using an Agilent catalog Probe Group. Also, if you prefer to increase the density of probes in the targeted genomic intervals, note that this will lead to the addition of probes that have lower scores. See FAQ “How many CGH probes and what density do I need to target a given genomic region?” (under "Creation of Probe Groups," above) for more details.

Create a microarray design from HD CGH/ChIP database probes (Wizard)

Before you use the wizard

To start the ChIP/CGH Wizard

Step 1 – HD Probe Search Details

Step 2 – HD Probe Search Submission

Step 3 – Create Probe Group

Step 4 – Define Design

Step 5 — Layout Probes

Step 6 — Create Microarray Design