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Expression monitoring to high density oligonucleotide arrays

a technology of oligonucleotide arrays and expression monitoring, which is applied in the field of expression monitoring to high density oligonucleotide arrays, can solve the problems of difficult or impossible differentiation of two or more gene products of approximately the same molecular weight, and the failure to provide an enabling method for using arrays of immobilized probes for this purpose, etc., and achieves small variations in expression levels.

Inactive Publication Date: 2005-09-15
AFFYMETRIX INC
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

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Benefits of technology

[0016] The pool of target nucleic acids can be the total polyA+ mRNA isolated from a biological sample, or cDNA made by reverse transcription of the RNA or second strand cDNA or RNA transcribed from the double stranded cDNA intermediate. Alternatively, the pool of target nucleic acids can be treated to reduce the complexity of the sample and thereby reduce the background signal obtained in hybridization. In one approach, a pool of mRNAs, derived from a biological sample, is hybridized with a pool of oligonucleotides comprising the oligonucleotide probes present in the high density array. The pool of hybridized nucleic acids is then treated with RNase A which digests the single stranded regions. The remaining double stranded hybridization complexes are then denatured and the oligonucleotide probes are removed, leaving a pool of mRNAs enhanced for those mRNAs complementary to the oligonucleotide probes in the high density array.
[0019] It will be appreciated that the methods of this invention can be used to monitor (detect and / or quantify) the expression of any desired gene of known sequence or subsequence. Moreover, these methods permit monitoring expression of a large number of genes simultaneously and effect significant advantages in reduced labor, cost and time. The simultaneous monitoring of the expression levels of a multiplicity of genes permits effective comparison of relative expression levels and identification of biological conditions characterized by alterations of relative expression levels of various genes. Genes of particular interest for expression monitoring include genes involved in the pathways associated with various pathological conditions (e.g., cancer) and whose expression is thus indicative of the pathological condition. Such genes include, but are not limited to the HER2 (c-erbB-2 / neu) proto-oncogene in the case of breast cancer, receptor tyrosine kinases (RTKs) associated with the etiology of a number of tumors including carcinomas of the breast, liver, bladder, pancreas, as well as glioblastomas, sarcomas and squamous carcinomas, and tumor suppressor genes such as the P53 gene and other “marker” genes such as RAS, MSH2, MLH1 and BRCA1. Other genes of particular interest for expression monitoring are genes involved in the immune response (e.g., interleukin genes), as well as genes involved in cell adhesion (e.g., the integrins or selectins) and signal transduction (e.g., tyrosine kinases), etc.
[0031]“Bind(s) substantially” refers to complementary hybridization between a probe nucleic acid and a target nucleic acid and embraces minor mismatches that can be accommodated by reducing the stringency of the hybridization media to achieve the desired detection of the target polynucleotide sequence.

Problems solved by technology

Others have proposed the use of large numbers of oligonucleotide probes to provide the complete nucleic acid sequence of a target nucleic acid but failed to provide an enabling method for using arrays of immobilized probes for this purpose.
The use of “traditional” hybridization protocols for monitoring or quantifying gene expression is problematic.
For example two or more gene products of approximately the same molecular weight will prove difficult or impossible to distinguish in a Northern blot because they are not readily separated by electrophoretic methods.
Similarly, as hybridization efficiency and cross-reactivity varies with the particular subsequence (region) of a gene being probed it is difficult to obtain an accurate and reliable measure of gene expression with one, or even a few, probes to the target gene.
In addition, the prior art provided no rapid and effective method for identifying a set of oligonucleotide probes that maximize specific hybridization efficacy while minimizing cross-reactivity nor of using hybridization patterns (in particular hybridization patterns of a multiplicity of oligonucleotide probes in which multiple oligonucleotide probes are directed to each target nucleic acid) for quantification of target nucleic acid concentrations.

Method used

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  • Expression monitoring to high density oligonucleotide arrays
  • Expression monitoring to high density oligonucleotide arrays
  • Expression monitoring to high density oligonucleotide arrays

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example 1

Detection of the Expression Levels of Target Genes

[0143] Experiments were designed to evalutate the specificity of hybridization, the relationship between hybridization signal and concentration of target nucleic acid, and the quantifiability of RNA detection at low concentration levels. These experiments involved hybridizing labeled RNA from a number of preselected genes (IL-2, IL-3, IL-4, IL-6, IL-10, IL-12p40, GM-CSF, IFN-γ, TNF-α, mCTLA8, β-actin, GAPDH, IL-11 receptor, and Bio B) to a high density oligonucleotide probe array comprising a large number of probes complementary to subsequences of these genes (see, Section B, below for a description of the array) in the presence or absence of an RNA sample transcribed from a cDNA library. The target genes were hybridized to the high density probe array either individually, together, or individually or together in the presence of labeled RNA transcribed from a murine cDNA library as described below.

[0144] A) Preparation of Labeled R...

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Abstract

This invention provides methods of monitoring the expression levels of a multiplicity of genes. The methods involve hybridizing a nucleic acid sample to a high density array of oligonucleotide probes where the high density array contains oligonucleotide probes complementary to subsequences of target nucleic acids in the nucleic acid sample. In one embodiment, the method involves providing a pool of target nucleic acids comprising RNA transcripts of one or more target genes, or nucleic acids derived from the RNA transcripts, hybridizing said pool of nucleic acids to an array of oligonucleotide probes immobilized on surface, where the array comprising more than 100 different oligonucleotides and each different oligonucleotide is localized in a predetermined region of the surface, the density of the different oligonucleotides is greater than about 60 different oligonucleotides per 1 cm2, and the olignucleotide probes are complementary to the RNA transcripts or nucleic acids derived from the RNA transcripts; and quantifying the hybridized nucleic acids in the array.

Description

BACKGROUND OF THE INVENTION [0001] Many disease states are characterized by differences in the expression levels of various genes either through changes in the copy number of the genetic DNA or through changes in levels of transcription (e.g. through control of initiation, provision of RNA precursors, RNA processing, etc.) of particular genes. For example, losses and gains of genetic material play an important role in malignant transformation and progression. These gains and losses are thought to be “driven” by at least two kinds of genes. Oncogenes are positive regulators of tumorgenesis, while tumor suppressor genes are negative regulators of tumorgenesis (Marshall, Cell, 64: 313-326 (1991); Weinberg, Science, 254: 1138-1146 (1991)). Therefore, one mechanism of activating unregulated growth is to increase the number of genes coding for oncogene proteins or to increase the level of expression of these oncogenes (e.g. in response to cellular or environmental changes), and another is...

Claims

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Application Information

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Patent Type & Authority Applications(United States)
IPC IPC(8): C12N15/09C12Q1/68G01N15/14G01N37/00G01N33/53
CPCC12Q1/6809C12Q1/6837G01N15/1475C12Q2565/507G01N15/1433
Inventor LOCKHART, DAVID J.BROWN, EUGENE L.WONG, GORDON G.CHEE, MARKGINGERAS, THOMAS R.
Owner AFFYMETRIX INC
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