Dr. Julio Fernández

FACULTY

RESEARCH

Ph.D. PROGRAM

M.A. BIOTECHNOLOGY

UNDERGRADUATE

COURSES



		FACULTY

			Faculty Interests
			Faculty Directory

FACULTY BIOGRAPHY

<-- Back

Julio M. Fernández

Professor

Lab Website

Classes:

W4510 : MOLECULAR SYSTEMS BIOLOGY I (Fall 2007)

W3008 : CELLULAR PHYSIOLOGY OF DISEASE (Spring 2007)

W4070 : BIOLOGY & PHYSICS OF SINGLE MOLECULES (Fall 2006)

C1000: FRONTIERS OF SCIENCE - Lecture/seminar (Spring 2006)

Recent Publications:

Wiita, A.P. et al, (2007) Probing the chemistry of thioredoxin catalysis with force. Nature , (in press).

Walther KA et al, (2007) Signatures of hydrophobic collapse in extended proteins captured with force spectroscopy Proc Natl Acad Sci U S A. 104:7916-21.

Brujic, J., (2006) Single molecule force spectroscopy reveals signatures of glassy dynamics in the energy landscape of ubiquitin. Nature Physics 2(4):282-286

Fernandez, J.M. and Li, H. B. Force-clamp spectroscopy monitors the folding trajectory of a single protein (2004), Science , 303: 1674-1678

Li, H. et al, (2002) Reverse engineering of the giant muscle protein titin . Nature , 418: 998-1002.

Research Topics:

The mechanical design of titin:
The protein titin provides muscle with its passive elasticity. Each titin molecule extends over half a sarcomere, and its extensibility has been studied both in situ6–10 and at the level of single molecules11–14. These studies suggested that titin is not a simple entropic spring but has a complex structure dependent elasticity. We use protein engineering and single molecule atomic force microscopy to examine the mechanical components that form the elastic region of human cardiac titin. We show that when these mechanical elements are combined, they explain the macroscopic behavior of titin in intact muscle. Our studies show the functional reconstitution of a protein from the sum of its parts.

The mechanical architecture of proteins:
One big advantage of our approach is that denaturing forces and extension can be controlled not only in magnitude but also in their direction. For example, we discovered that the mechanical stability and unfolding pathway of ubiquitin strongly depend on the linkage through which the mechanical force is applied to the protein. Hence, a protein that is otherwise very stable may be easily unfolded by a relatively weak mechanical force applied through the right linkage. This may be a widespread mechanism in biological systems. Another surprising finding was the discovery that ankyrin, a protein made of multiple repeats, upon pulling, unfolds in a piecewise manner. The piecewise unfolding of multiple ANK repeats could behave like multiple buffers linked in series; to resist damagingly high forces, ANK repeats can be sacrificed and extended one at a time, without the whole protein losing its tertiary structure. Both of these discoveries are completely novel and could not have been anticipated from solution biochemistry.

Studies of protein folding from highly extended states:
Force-clamp spectroscopy is a novel platform to study protein folding. The coordinate for the unfolding reaction is known (end-to-end length), the unfolded state is well defined and can be controlled over wide ranges, and the folding trajectory can be followed in a single protein over time. We use two force-clamp protocols: force-quench and force-ramp. In contrast to the traditional two-state folding reactions observed in solution biochemistry, our folding trajectories from highly extended unfolded states are continuous and marked by several distinct stages. The time taken to fold is exponentially dependent on the stretching force applied during folding. While chain entropy makes a small contribution to the collapse, we have found that most of the driving force is hydrophobic and varying widely depending on the dihedral space traversed by the folding trajectory. This collapse mechanism is common to highly extended proteins, including non-folding elastomeric proteins like PEVK from titin.

Chemical reactions under a stretching force:
The mechanism by which mechanical forces regulate the kinetics of a chemical reaction is unknown. We use single molecule force-clamp spectroscopy and protein engineering to study the effect of force on the kinetics of thiol/disulfide exchange. Reduction of disulfide bonds via the thiol/disulfide exchange chemical reaction is crucial in regulating protein function and is of common occurrence in mechanically stressed proteins. Our work at the single bond level directly demonstrates that thiol/disulfide exchange in proteins is a force-dependent chemical reaction. Our findings suggest that mechanical force plays a role in disulfide reduction in vivo, a property which has never been explored by traditional biochemistry. Furthermore, our work also suggests that the kinetics of any chemical reaction that results in bond lengthening will be force dependent.

Enzyme catalysis under force:
Thioredoxins are enzymes that catalyze disulfide bond reduction in all living organisms. While catalysis is thought to proceed through a substitution nucleophilic bimolecular (SN2) reaction, the role of the enzyme in modulating this chemical reaction is unknown. Here we use single molecule force-clamp spectroscopy to probe the catalytic mechanism of E. coli thioredoxin (Trx). We apply mechanical force in the range of 25-450 pN to a disulfide bond substrate and monitor the reduction of these bonds by individual enzymes. Our results suggest that substrate conformational changes may be important in the regulation of Trx activity under conditions of oxidative stress and mechanical injury, such as those experienced in cardiovascular disease. Furthermore, single molecule atomic force microscopy (AFM) techniques, as shown here, can probe dynamic rearrangements within an enzyme's active site which cannot be resolved with any other current structural biological technique.

Representative Recent Publications

Brujic, J., Hermans, R.I., Walther, K.A. and Julio M. Fernandez (2006) Single molecule force spectroscopy reveals signatures of glassy dynamics in the energy landscape of ubiquitin Nature Physics 2(4): 282-286. Article
Wiita, A.P., Ainavarapu, S.R.K., Huang, H.H. and Julio M. Fernandez (2006) Force dependent chemical kinetics of disulfide bond reduction observed with single molecule techniques Proc Natl Acad Sci USA 103(19): 7222-7. Article
Fernandez, J.M. and Li, H. B (2004) Force-clamp spectroscopy monitors the folding trajectory of a single protein Science 303: 1674-1678. Article
Carrion-Vazquez, M.; Li, H.; Lu, H.; Marszalek, P. E.; Oberhauser, A. F.; Fernandez, J. M (2003) The mechanical stability of ubiquitin is linkage dependent Nature Structural Biology 10(9): 738-43. Article
Li, H. B.; Linke, W. A.; Oberhauser, A. F.; Carrion-Vazquez, M.; Kerkvliet, J. G.; Lu, H.; Marszalek, P. E.; Fernandez, J. M (2002) Reverse engineering of the giant muscle protein titin Nature 418: 998-1002. Article
Li, H., Carrion-Vazquez, M., Oberhauser, A.F., Marszalek, P.E. and Fernandez, J.M (2000) Point mutations alter the mechanical stability of immunoglobulin modules Nature Structural. Biology 7(12): 1117-1120. Article
Marszalek, P.E., Lu, H., Li, H., Carrion-Vazquez, M., Oberhauser, A.F., Schulten, K. and Fernandez, J.M (1999) Mechanical unfolding intermediates in titin modules Nature 402: 100-103. Article
Oberhauser, A.F., Marszalek, P.E., Carrion-Vazquez, M., and Fernandez, J.M (1999) Single protein misfolding events captured by atomic force microscopy Nature Struct.Biol 6: 1025-1028. Article
Carrion-Vazquez, M., Oberhauser, A.F., Fowler, S.B., Marszalek, P.E., Broedel, S.E.,Clarke, J., and Fernandez, J.M. (1999) Mechanical and chemical unfolding of a single protein: a comparison. Proc. Natl. Acad. Sci 96: 3694-3699. Article
Marszalek, P.M., Oberhauser, A.F., Pang, Y.-P., and Fernandez, J.M. (1998) Polysaccharide elasticity governed by chair-boat transitions of the glucopyranose ring Nature 396: 661-664. Article
Oberhauser, A.F., Marszalek, P.E., Erickson, H.P., and Fernandez, J.M (1998) The molecular elasticity of tenascin, an extracellular matrix protein Nature 393: 181-185. Article
Rief, M., Gautel, M., Oesterhelt, F., Fernandez, J.M. and Gaub, H.E (1997) Reversible unfolding of individual titin immunoglobulin domains by AFM Science 276: 1109-1112. Article
Rahamimoff, R., and Fernandez, J.M (1997) Pre-and postfusion regulation of transmitter release Neuron 18: 17-27.
Robinson, I.M., Finnegan, J.M., Monck, J.R., Wightman, R.M. and Fernandez, J.M (1995) Colocalisation of calcium entry and exocytotic release sites in adrenal chromaffin cells Proc. Natl. Acad. Sci USA 92: 2474-2478. Article
Escobar, A.L., Monck, J.R., Fernandez, J.M. and Vergara, J.L (1994) Localization of the site of Ca2+ release at the level of a single sarcomere in skeletal muscle fibers Nature 367: 739-741.
Nanavati, C., and Fernandez, J.M. (1993) The secretory granule matrix: a fast acting smart polymer Science 259: 963-965. Article
Monck, J.R., Alvarez de Toledo, G. and Fernandez, J.M (1990) Tension in secretory granule membranes causes extensive membrane transfer through the exocytotic fusion pore Proc. Natl. Acad. Sci 87: 7804-7808. Article
Lindau, M. and Fernandez, J.M. (1986) IgE-mediated degranulation of mast cells does not require opening of ion channels Nature 319: 150-153. Article
Schroeder, J.I., Hedrich, R. and Fernandez, J.M. (1984) Potassium-selective single channels in guard cell protoplast of Vicia faba Nature 312: 361-362. Article
Fernandez, J.M., Neher, E. and Gomperts, B.D. (1984) Capacitance measurements reveal stepwise fusion events in degranulating mast cells Nature 312: 453-455. Article





	Columbia University Biological Sciences
	1011A Fairchild Center MC 2449 New York, NY 10027 Phone office: (212) 854-9141 lab: (212) 854-9474 fax: (212) 854-4619 Email jf2120@columbia.edu Lab Directory