Distinguishing PCA3 messenger RNA species in benign and malignant prostate tissues
First Claim
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1. A method of determining the malignancy status of prostate cells contained in a sample undergoing testing, said method comprising:
- (a) amplifying PCA3 nucleic acids using RNA templates and a pair of oligonucleotides which amplify across nucleotide positions 26 and 255 of SEQ ID NO;
1 and across nucleotide positions 26 and 27 of SEQ ID NO;
2, thereby resulting in a collection of amplified nucleic acids, when said PCA3 nucleic acids are present, said collection comprising(i) a PCA3 nucleic acid that comprises an additional sequence between PCA3 exon 3 and PCA3 exon 4a, said additional sequence consisting essentially of nucleotides 27 to 254 of SEQ ID NO;
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(ii) a PCA3 nucleic acid that comprises PCA3 exon 3 joined to PCA3 exon 4a without including said additional sequence; and
(b) detecting among said collection of amplified nucleic acids(iii) substantially only said PCA3 nucleic acid that comprises PCA3 exon 3 joined to PCA3 exon 4a without including said additional sequence, and not said PCA3 nucleic acid that comprises said additional sequence, if said sample comprises prostate cancer cells; and
(iv) substantially only said PCA3 nucleic acid that comprises said additional sequence between PCA3 exon 3 and PCA3 exon 4a, and not said PCA3 nucleic acid that comprises PCA3 exon 3 joined to PCA3 exon 4a without including said additional sequence, if prostate cells contained in the sample consist of benign prostate cells associated with BPH,thereby determining the malignancy status of prostate cells contained in said sample.
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Abstract
This invention concerns the discovery of two distinct PCA3 mRNA sequences. One of these sequences corresponds to a short PCA3 mRNA molecule whereas the other PCA3 RNA molecule is longer as it comprises an additional sequence between exon 3 and exon 4a. The short RNA is associated with prostate cancer whereas the long RNA sequence is associated with a non-malignant state of the prostate. Based on the differential expression levels of these two PCA3 RNA sequences, protocols for the diagnosis of prostate disease are provided. The invention also relates to therapeutic approaches to prostate cancer.
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Citations
20 Claims
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1. A method of determining the malignancy status of prostate cells contained in a sample undergoing testing, said method comprising:
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(a) amplifying PCA3 nucleic acids using RNA templates and a pair of oligonucleotides which amplify across nucleotide positions 26 and 255 of SEQ ID NO;
1 and across nucleotide positions 26 and 27 of SEQ ID NO;
2, thereby resulting in a collection of amplified nucleic acids, when said PCA3 nucleic acids are present, said collection comprising(i) a PCA3 nucleic acid that comprises an additional sequence between PCA3 exon 3 and PCA3 exon 4a, said additional sequence consisting essentially of nucleotides 27 to 254 of SEQ ID NO;
1; and(ii) a PCA3 nucleic acid that comprises PCA3 exon 3 joined to PCA3 exon 4a without including said additional sequence; and (b) detecting among said collection of amplified nucleic acids (iii) substantially only said PCA3 nucleic acid that comprises PCA3 exon 3 joined to PCA3 exon 4a without including said additional sequence, and not said PCA3 nucleic acid that comprises said additional sequence, if said sample comprises prostate cancer cells; and (iv) substantially only said PCA3 nucleic acid that comprises said additional sequence between PCA3 exon 3 and PCA3 exon 4a, and not said PCA3 nucleic acid that comprises PCA3 exon 3 joined to PCA3 exon 4a without including said additional sequence, if prostate cells contained in the sample consist of benign prostate cells associated with BPH, thereby determining the malignancy status of prostate cells contained in said sample. - View Dependent Claims (2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17)
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18. A method of distinguishing differentially expressed PCA3 nucleic acids that indicate the malignancy status of prostate cells contained in a sample undergoing testing, said method comprising:
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(a) performing a nucleic acid amplification reaction, using RNAs obtained from prostate cells contained in said sample as templates to amplify PCA3 nucleic acid sequences across nucleotide positions 26 and 255 of SEQ ID NO;
1, which respectively define the PCA3 exon 3-intron 3 and intron 3-exon 4a junctions, and nucleotide positions 26 and 27 of SEQ ID NO;
2, which define the PCA3 exon 3-exon 4a junction, whereby there are synthesized first and second amplification products;wherein said first amplification product results from an amplification of a first PCA3 RNA that comprises portions of exon 3 and exon 4a sequences and an additional sequence between PCA3 exon 3 and PCA3 exon 4a, said additional sequence consisting essentially of nucleotides 27 to 254 of SEQ ID NO;
1, andwherein said second amplification product results from an amplification of a second PCA3 RNA that comprises portions of exon 3 and exon 4a sequences with PCA3 exon 3 joined to PCA3 exon 4a without including said additional sequence; and (b) detecting one of said first and second amplification products independent of the other, thereby distinguishing differentially expressed PCA3 nucleic acids that indicate the status of prostate cells contained in said sample. - View Dependent Claims (19)
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20. A kit for determining the malignancy status of prostate cells by distinguishing between a non-malignant PCA3 nucleic acid and a malignant PCA3 nucleic acid in a sample undergoing testing said kit comprising:
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(a) a pair of oligonucleotides which amplify across nucleotide positions 26 and 255 of SEQ ID NO;
1 and across nucleotide positions 26 and 27 of SEQ ID NO;
2, thereby resulting in a collection of amplified nucleic acids, when said PCA3 nucleic acids are present, said collection comprising a PCA3 nucleic acid that comprises an additional sequence between PCA3 exon 3 and PCA3 exon 4a, said additional sequence consisting essentially of nucleotides 27 to 254 of SEQ ID NO;
1, and a PCA3 nucleic acid that comprises PCA3 exon 3 joined to PCA3 exon 4a without including said additional sequence; and(b) a probe hybridizing under high stringency conditions to at least 10 consecutive nucleotides of a nucleic acid comprising nucleotide positions 26 and 27 of SEQ ID NO;
2, which define the PCA3 exon 3-exon 4a junction, thereby detecting among said collection of amplified nucleic acids substantially only said PCA3 nucleic acid that comprises PCA3 exon 3 joined to PCA3 exon 4a without including said additional sequence, and not said PCA3 nucleic acid that comprises said additional sequence.
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Specification