Jesse J Salk

7632642, Dec 15, 2009

Oct 17, 2005

11/252433

Lawrence J. Wangh - Auburndale MA, US
John Rice - Quincy MA, US
J. Aquiles Sanchez - Framingham MA, US
Kenneth Pierce - Natick MA, US
Jesse Salk - Seattle WA, US
Arthur Reis - Arlington MA, US
Cristina Hartshorn - Needham MA, US

Brandeis University - Waltham MA

C12Q 1/68
C12P 19/34
C07H 21/04

435 6, 435 912, 536 243

Homogenous detection during or following PCR amplification, preferably LATE-PCR, utilizing fluorescent DNA dye and indirectly excitable labeled primers and probes, improves reproducibility and quantification. Low-temperature homogeneous detection during or following non-symmetric PCR amplification, preferably LATE-PCR, utilizing fluorescent DNA dye and indirectly excitable labeled mismatch-tolerant probes permits analysis of complex targets. Sequencing sample preparation methods following LATE-PCR amplifications reduce complexity and permit “single-tube” processing.

20060177842, Aug 10, 2006

Oct 17, 2005

11/252506

Lawrence Wangh - Auburndale MA, US
John Rice - Quincy MA, US
J. Sanchez - Framingham MA, US
Kenneth Pierce - Natick MA, US
Jesse Salk - Seattle WA, US
Arthur Reis - Arlington MA, US
Cristina Hartshorn - Needham MA, US

C12Q 1/68
C07H 21/04
C12P 19/34

435006000, 435091200, 536024100

An additive for preventing mispriming in polymerase chain reaction (PCR) amplifications and assays comprising a hairpin oligonucleotide having a stem duplex greater than six nucleotides in length and a stabilized stem terminus. The additive improves PCR amplifications, including LATE-PCR amplifications when added to initial amplification reaction mixtures. It can be included in oligonucleotide sets and in kits for PCR amplification and assays.

20090226973, Sep 10, 2009

Mar 20, 2009

12/382670

Lawrence J. Wangh - Auburndale MA, US
John Rice - Quincy MA, US
J. Aquiles Sanchez - Framingham MA, US
Kenneth Pierce - Natick MA, US
Jesse Salk - Seattle WA, US
Arthur Reis - Arlington VA, US
Cristina Hartshorn - Needham MA, US

C12P 19/34
C07H 21/00
C12N 9/00

435 912, 536 221, 435183

An additive for preventing mispriming in polymerase chain reaction (PCR) amplifications and assays comprising a hairpin oligonucleotide having a stem duplex greater than six nucleotides in length and a stabilized stem terminus. The additive improves PCR amplifications, including LATE-PCR amplifications when added to initial amplification reaction mixtures. It can be included in oligonucleotide sets and in kits for PCR amplification and assays.

20110003289, Jan 6, 2011

Mar 17, 2010

12/726287

Jesse Salk - Seattle WA, US
Stephen Salipante - Seattle WA, US

University of Washington - Seattle WA

C12Q 1/68
C07H 21/00

435 6, 536 2433

Among other aspects, the present invention provides biomarkers and methods of identifying precancerous fields in a subject in need thereof. Methods of diagnosing and for providing a prognosis for a subject with an increased risk of developing cancer are also provided, along with methods of determining surgical margins for a tumor or tissue resection procedure. Additionally, reagents and kits are provided for the practice of the methods disclosed herein.

20120040352, Feb 16, 2012

Nov 10, 2008

12/292038

Lawrence J. Wangh - Auburndale MA, US
John Rice - Quincy MA, US
J. Aquiles Sanchez - Framingham MA, US
Kenneth Pierce - Natick MA, US
Jesse Salk - Seattle WA, US
Arthur Reis - Arlington MA, US
Cristina Hartshorn - Needham MA, US

C12Q 1/68
C12P 19/34
C12N 9/00
C07H 21/04

435 612, 536 243, 536 2433, 435 912, 435183

Homogenous detection during or following PCR amplification, preferably LATE-PCR, utilizing fluorescent DNA dye and indirectly excitable labeled primers and probes, improves reproducibility and quantification. Low-temperature homogeneous detection during or following non-symmetric PCR amplification, preferably LATE-PCR, utilizing fluorescent DNA dye and indirectly excitable labeled mismatch-tolerant probes permits analysis of complex targets. Sequencing sample preparation methods following LATE-PCR amplifications reduce complexity and permit “single-tube” processing.

20130095479, Apr 18, 2013

Aug 1, 2012

13/564528

Lawrence J. Wangh - Auburndale MA, US
John Rice - Quincy MA, US
J. Aquilles Sanchez - Framingham MA, US
Kenneth Pierce - Natick MA, US
Jesse Salk - Seattle WA, US
Arthur Reis - Arlington MA, US
Cristina Hartshorn - Needham MA, US

BRANDEIS UNIVERSITY - Waltham MA

C12Q 1/68

435 611, 435 612

Homogenous detection during or following PCR amplification, preferably LATE-PCR, utilizing fluorescent DNA dye and indirectly excitable labeled primers and probes, improves reproducibility and quantification. Low-temperature homogeneous detection during or following non-symmetric PCR amplification, preferably LATE-PCR, utilizing fluorescent DNA dye and indirectly excitable labeled mismatch-tolerant probes permits analysis of complex targets. Sequencing sample preparation methods following LATE-PCR amplifications reduce complexity and permit “single-tube” processing.

20220267841, Aug 25, 2022

Apr 12, 2022

17/719147

- Seattle WA, US
Lawrence A. LOEB - Bellevue WA, US
Jesse J. SALK - Seattle WA, US

C12Q 1/6869
C12Q 1/6855

Disclosed herein are adapter nucleic acid sequences, double-stranded complexed nucleic acids, compositions, and methods for sequencing a double-stranded target nucleic acid with applications to error correction by duplex sequencing.

20220220543, Jul 14, 2022

Aug 1, 2020

17/607490

- Seattle WA, US
Jesse J. SALK - Seattle WA, US

C12Q 1/6827
C12Q 1/6869

The present technology relates generally to the methods and associated reagents for providing error-corrected nucleic acid sequences. In particular, several embodiments are directed to adapter molecules comprising a hairpin shape and methods of use of such adapters in Duplex Sequencing and other sequencing applications. In some embodiments, physically-linked nucleic acid complexes comprising both the first strand and the second strand can be amplified and independently sequenced in a same clonal cluster on a sequencing surface.