Norman Arnheim scite author profile

Two new methods were used to establish a rapid and highly sensitive prenatal diagnostic test for sickle cell anemia. The first involves the primer-mediated enzymatic amplification of specific beta-globin target sequences in genomic DNA, resulting in the exponential increase (220,000 times) of target DNA copies. In the second technique, the presence of the beta A and beta S alleles is determined by restriction endonuclease digestion of an end-labeled oligonucleotide probe hybridized in solution to the amplified beta-globin sequences. The beta-globin genotype can be determined in less than 1 day on samples containing significantly less than 1 microgram of genomic DNA.

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Most human carcinomas of the exocrine pancreas contain mutant c-K-ras genes

Almoguera

Shibata

Forrester

et al. 1988

Cell

1,927

1,046

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Involvement of mouse Mlh1 in DNA mismatch repair and meiotic crossing over

et al. 1996

Nat Genet

762

596

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Mice that are deficient in either the Pms2 or Msh2 DNA mismatch repair genes have microsatellite instability and a predisposition to tumours. Interestingly, Pms2-deficient males display sterility associated with abnormal chromosome pairing in meiosis. Here mice deficient in another mismatch repair gene, Mlh1, possess not only microsatellite instability but are also infertile (both males and females). Mlh1-deficient spermatocytes exhibit high levels of prematurely separated chromosomes and arrest in first division meiosis. We also show that Mlh1 appears to localize to sites of crossing over on meiotic chromosomes. Together these findings suggest that Mlh1 is involved in DNA mismatch repair and meiotic crossing over.

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Whole genome amplification from a single cell: implications for genetic analysis.

Zhang

Cui

Schmitt

et al. 1992

Proc. Natl. Acad. Sci. U.S.A.

813

523

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We have developed an in vitro method for amplifying a large fraction of the DNA sequences present in a single haploid cell by repeated primer extensions using a mixture of 15-base random oligonucleotides. We studied 12 genetic loci and estimate that the probability of amplifying any sequence in the genome to a minimum of 30 copies is not less than 0.78 (95% confidence). Whole genome amplification beginning with a single cell, or other samples with very small amounts of DNA, has significant implications for multipoint mapping by sperm or oocyte typing and possibly for genetic disease diagnosis, forensics, and the analysis of ancient DNA samples.

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Hydroxylated Quantum Dots as Luminescent Probes for in Situ Hybridization

et al. 2001

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Norman Arnheim

Enzymatic Amplification of β-Globin Genomic Sequences and Restriction Site Analysis for Diagnosis of Sickle Cell Anemia

Most human carcinomas of the exocrine pancreas contain mutant c-K-ras genes

Involvement of mouse Mlh1 in DNA mismatch repair and meiotic crossing over

Whole genome amplification from a single cell: implications for genetic analysis.

Hydroxylated Quantum Dots as Luminescent Probes for in Situ Hybridization

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