USDOE Human Subjects Research Database, Fiscal Year 1997

Department of Molecular Biology, Princeton University

Public Information Contact:

Dr. Jacques R. Fresco
Department of Molecular Biology
Princeton University
Princeton, NJ 08544

Phone: 609-258-3927
Fax: 609-258-1208
Email: jrfresco@princeton.edu

Institutional Review Board (IRB):

Projects are approved by an IRB located at: Princeton University.
The approving IRB operates under a Multiple Project Assurance (MPA) recognized by DOE or by the Department of Health and Human Services (HHS).
MPA number of the IRB:

Human Subjects Projects:

Number of Human Subjects Projects reported: 1

PU-96-DE-FG02-96ER62202

Development of Affinity Technology for Isolating Individual Human Chromosomes by Third Strand Binding

Project Identifier: PU-96-DE-FG02-96ER62202

Project Title:

Development of Affinity Technology for Isolating Individual Human Chromosomes by Third Strand Binding

Principal Investigator: Dr. Jacques R. Fresco
Principal Investigator's Institution: Department of Molecular Biology

Project started in: 1996

Fiscal Year 1997 Funding for Research on Human Subjects:

Project Funding Information:
Project received funding in Fiscal Year 1997.
Project used human subjects in Fiscal Year 1997.

Funding Sources:

DOE: Health Effects and Life Sciences Research Division, ER-72

Amount: $208,084
Comments:

Blood samples taken at the Princeton University Infirmary were provided by the principal investigator and the Ph.D. researcher of the grant, all at no cost

Information on Use of Human Subjects:

Project does not involve use of multiple protocols/subprojects.

IRB Review:
Type of Review: Full Board
Most Recent Approval: May 13, 1998

Number of Human Subjects who participated in this project/protocol during FY 1997 (10/1/96 - 9/30/97): 2

Type of Human Subjects Involvement:

Collection of Bodily Materials:

Collection of personally identifiable bodily materials (blood or blood products, cells, tissue, organs, waste).

• Use of cells cultured in a laboratory.
• Use of bodily materials collected from subjects specifically for this project.

(a. Objectives, b. Methodology, c. Ionizing Radiation, Radioactive Substances, or Chemical Substances to which human subjects are exposed, d. Involvement of Human Subjects [d.1. procedures used, d.2. risks if any])

A. OBJECTIVE

The aim of this project is to exploit "third-strand" nucleic acid binding, which involves non-denaturing conditions, to target duplexes for the purpose of developing new technologies for chromosome identification, sorting, and bulk isolation. The respective technologies, triplex in situ hybridization (TISH), triplex univariate flow sorting, and triplex affinity chromosome purification, depend on the design of nucleic acid third-strands to bind with great specificity and affinity via triple helix formation to repetitive double helical centromeric alpha satellite DNA target sequences unique to individual human chromosomes.

A single copy of the alphoid DNA target sequence is present within each tandemly repeated higher order alpha-satellite DNA array. These arrays, are, in turn, located in an anatomically unique chromosomal region, the centromere, where they are likely to be more accessible to third-strand binding than endogenous hetero-and euchromatin. Moreover, target sequences for third-strand binding have a high probability of being chromosome-specific since alphoid DNAs differ with respect to their degree of sequence relatedness.

B. METHODOLOGY

We outline below the generic approach that should allow third-strand probes to bind to any human metaphase chromosome in situ and in suspension.

1. Selection of a centromeric alphoid DNA target sequence that is unique to a particular human chromosome and present in multiple copies. A database search has confirmed the presence of unique alpha-satellite target sequences in 21 of the 24 human chromosomes.

2. Design of oligodeoxynucleotide third-strand affinity probes for binding to alphoid DNA target sequences.

3. Determination that the third-strand affinity probes can bind specifically to their alphoid DNA target sequences in recombinant DNA molecules under buffer conditions optimal for chromosome hybridization.

4. Confirmation by Triplex In Situ Hybridization (TISH) of third-strand binding to duplex alphoid DNA targets on metaphase chromosome spreads from cultured human lymphocytes.

5. Development of Triplex Suspension Hybridization (TSH), and if necessary, gentle extraction procedures to remove centromere-bound proteins.

6. Determination of ability of biotinylated third strands to affinity capture the correct metaphase chromosome from a suspension using different streptavidin-based approaches.

7. Determination of conditions for bulk isolation and purification of the correct metaphase chromosome by third strand affinity capture.

C. IONIZING RADIATION, RADIOACTIVE SUBSTANCES, CHEMICAL SUBSTANCES

Not applicable.

D. INVOLVEMENT OF HUMAN SUBJECTS

No statistical sample data collection is involved. A few healthy human blood donors from our own research group donate 10 ml of blood, drawn at the Princeton University Infirmary under standard sterile conditions. Aliquots of this blood are cultured under standard sterile conditions in order to obtain metaphase and interphase lymphocytes for cytogenetic analysis. There are no risks to human donors, and all subsequent studies are performed in vitro. No public references to sources of donors are planned; and blood samples are volunteered by the researchers themselves.