Integrated Membrane for Preservation of Biomolecules

Abstract

An apparatus and method for moiety specific sample extraction from a complex sample matrix in a flow through process is provided. The present invention relates to an integrated membrane for separation and preservation of biomolecules. Classes of biomolecules, for example, those in blood, can be separated and preserved. For blood separation, the apparatus includes a housing having a matrix portion, and a fluid collection portion disposed within an inner cavity thereof. The housing also includes an aperture permitting access to the inner cavity. The apparatus also includes a matrix disposed within the matrix portion. The matrix includes a first layer for collecting substantially all cells from the fluid, a second layer for protein adsorption, and a third layer for nucleic acid adsorption. Fluid enters the housing through the aperture, passes through the matrix, and into the fluid collection portion. The method includes passing fluid through a matrix; collecting substantially all cells from the fluid in a layer of the matrix; adsorbing protein from the fluid in a layer of the matrix; and adsorbing nucleic acid from the fluid in a layer of the matrix.

Description

[0001]This application is a non-provisional patent application claiming priority to U.S. provisional patent application No. 61 / 685,330 filed on Mar. 14, 2012, entitled “An integrated membrane for the preservation of biomolecules utilizing membrane-adsorbent technology to autonomously fractionate and preserve proteins and nucleic acids for long-term storage at conditions” incorporated by reference herein.[0002]This invention was made under a contract with an agency of the U.S. Government, Army Phase I Contract No: W81XWH-12-C-0002.FIELD OF THE DISCLOSURE[0003]The present invention relates to an apparatus and method for moiety specific sample extraction from a complex sample matrix in a flow through process. An integrated membrane is used for separation and preservation of biomolecules. Classes of biomolecules, such as those in blood, can be separated and preserved.BACKGROUND[0004]The present invention relates to separation and analysis of biomolecules, especially those of bodily flui...

AI Technical Summary

Benefits of technology

The patent discusses a method for extracting samples from cells without causing degradation of the substances being analyzed. This is done by using special buffers to lyse the cells and separate the samples. The process is fast, and helps to protect the quality of the samples. The patent also mentions a special membrane that is used to quickly process samples and prevent degradation. Overall, this method allows for more efficient and accurate analysis of samples from cells.

Problems solved by technology

These procedures typically require considerable care and attention.

For example, the storage of highly labile biomolecules, such as proteins and RNA, requires the use of low (4° C. and −20° C.) and ultra-low (−80° C.) freezers and / or a host of specialized and expensive chemicals to preserve the structural and chemical integrity of the biomolecule.

Because of these storage requirements, storing millions of samples to use for early diagnosis is cost prohibitive and impractical.

Presently, alternatives to low and ultra-low temperature storage have significant drawbacks.

Because RNases are ubiquitous in the clinic and laboratory, clinicians are unable to institutionalize reliable procedures for avoiding contamination.

While these reagents theoretically provide for the storage of RNA samples at near room temperature for up to seven (7) days, actual use shows that there is significant mRNA degradation that may occur after three (3) days of near-room temperature storage.

With regard to protein storage, there is currently no commercially available means of storage other than the low and ultra-low temperature methodology.

Alternative methodologies exist but are deficient.

Current DBS technology is limited and an inferior substitute for low and ultra-low temperature storage of samples.

Special training of personnel handling the placement of the blood on the papers / cards is required or large variations and errors can result.

For example, DBS papers in use are subject to operator inefficiencies and lack of skill.

Operator errors in the distribution of the samples on the matrix is often non-uniform, leading to assay variations (upon recovery).

And, samples are recovered using a punch device, which can lead to cross-contamination among samples.

Images