Structure and mechanics of proteins from single molecules to cells.

Format:

Book

Thesis/Dissertation

Author/Creator:

Brown, Andre E.

Contributor:

Discher, Dennis E. (Dennis Edward), advisor.

University of Pennsylvania.

Language:

English

Subjects (All):

Biophysics.

Physics.

Mechanical engineering.

Biomedical engineering.

0541.

0548.

0605.

0786.

Penn dissertations--Physics and astronomy.

Physics and astronomy--Penn dissertations.

Local Subjects:

Penn dissertations--Physics and astronomy.

Physics and astronomy--Penn dissertations.

0541.

0548.

0605.

0786.

Physical Description:

131 pages

Contained In:

Dissertation Abstracts International 71-04B.

System Details:

Mode of access: World Wide Web.

text file

Summary:

Physical factors drive evolution and play important roles in motility and attachment as well as in differentiation. As animal cells adhere to survive, they generate force and "feel" various mechanical features of their surroundings and respond to externally applied forces. This mechanosensitivity requires a substrate for cells to adhere to and a mechanism for cells to apply force, followed by a cellular response to the mechanical properties of the substrate. We have taken an outside-in approach to characterize several aspects of cellular mechanosensitivity. First, we used single molecule force spectroscopy to measure how fibrinogen, an extracellular matrix protein that forms the scaffold of blood clots, responds to applied force and found that it rapidly unfolds in 23 nm steps at forces around 100 pN. Second, we used tensile testing to measure the force-extension behavior of fibrin gels and found that they behave almost linearly to strains of over 100%, have extensibilities of 170 +/- 15%, and undergo a large volume decrease that corresponds to a large and negative peak in compressibility at low strain, which indicates a structural transition. Using electron microscopy and X-ray scattering we concluded that these properties are likely due to coiled-coil unfolding, as observed at the single molecule level in fibrinogen. Moving inside cells, we used total internal reflection fluorescence and atomic force microscopy to image self-assembled myosin filaments. These filaments of motor proteins that are responsible for cell and muscle contractility were found to be asymmetric, with an average of 32% more force generating heads on one half than the other. This could imply a force imbalance, so that rather than being simply contractile, myosin filaments may also be motile in cells.

Notes:

Thesis (Ph.D. in Physics and Astronomy) -- University of Pennsylvania, 2009.

Source: Dissertation Abstracts International, Volume: 71-04, Section: B, page: 2437.

Adviser: Dennis E. Discher.

Local Notes:

School code: 0175.

ISBN:

9781109709209

Access Restriction:

Restricted for use by site license.