Can High Pressures Enhance The Long-Term Survival of Microorganisms? Can High Pressures Enhance The Long-Term Survival of Microorganisms? Robert M. Hazen.

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Presentation transcript:

Can High Pressures Enhance The Long-Term Survival of Microorganisms? Can High Pressures Enhance The Long-Term Survival of Microorganisms? Robert M. Hazen & Matt Schrenk Carnegie Institution & NASA Astrobiology Institute Pardee Keynote Symposium: Evidence for Long-Term Survival of Microorganisms and Preservation of DNA Philadelphia – October 24, 2006

ObjectivesObjectives Review the nature and distribution of life at high pressures. I. Review the nature and distribution of life at high pressures. II. Examine the extreme pressure limits of cellular life. III. Compare experimental approaches to study microbial behavior at high P and T. IV. Explore how biomolecules and their reactions might change at high pressure?

I. High-Pressure Life HMS Challenger – 1870s 20 MPa (~200 atmospheres)

High-Pressure Life Deep-Sea Hydrothermal Vents – 1977

High-Pressure Life Discoveries of Microbial Life in Crustal Rocks – 1990s P ~ 100 MPa

Witwatersrand Deep Microbiology Project Energy from radiolytic cleavage of water. Lin, Onstott et al. (2006) Science

Thomas Gold’s Hypothesis: Organic Synthesis in the Mantle Thomas Gold (1999) NY:Springer-Verlag.  >300 MPa

Life at High Pressures on other Worlds? Life at High Pressures on other Worlds? Deep, wet environments may exist on Mars, Europa, etc.

I. What is the Nature and Distribution of Life at High-Pressure? Deep life, especially microbial life, is abundant throughout the upper crust. Deep life, especially microbial life, is abundant throughout the upper crust.

II. What are the Extreme Pressure Limits of Life? How deep might microbes exist in Earth’s crust?

Pressure Can Enhance T Stability [Margosch et al. (2006) Appl. Environ. Microbiology 72, ] [Pledger et al. (1994) FEMS Microbiology Ecology 14, ]

Life’s Extreme Pressure Limits Fast, cold slabs have regions of P > 2 GPa & T < 150°C [Stein & Stein (1996) AGU Monograph 96] 60 km

Hydrothermal Opposed-Anvil Cell Pressure Limits of Life

Microbes and their environment can be probed optically at pressure. [Sharma et al. (2002) Science 295, ] E. coli 1 atm 1.4 GPa 1 hour 1.4 GPa >30 hours

Pressure Limits of Life Ice VI forms at P > 1.0 GPa & 25°C. Microbes persist at triple junctions [Sharma et al. (2002) Science 295, ] E. coli 1 atm 1.4 GPa 1 hour 1.4 GPa >30 hours

Pressure Limits of Life Raman measurements show formate reduction to P > 1.4 GPa. Microbes shape their icy environment and viable microbes are recovered after several days at 1.4 GPa & 25°C. [Sharma et al. (2002) Science 295, ] E. coli 1 atm 1.4 GPa 1 hour 1.4 GPa >30 hours

II. What are the Extreme Pressure Limits of Life? Some microbes survive at P > 1.4 GPa (~14,000 atm). Temperature limits are not known, but pressure enhances T-tolerance for some microbes.

Hydrothermal Opposed-Anvil Cell III. Techniques for Studying Microbes at High Pressure

High-Pressure Techniques Gold tube reactors in hydrothermal bombs

Flow-through Reactor [Jannasch et al. (1996) Appl. & Environ. Microbiology 62, ] High-Pressure Techniques

Flow-through Reactor High-Pressure Techniques

New Opposed Anvil Cell “Large” volume: 100 mm 3 at 200 MPa 10 mm 3 at 500 MPa Easy optical access Rapid loading Heating options Cryo-quenching Inexpensive Moissanite (SiC) anvils Four-screw design Aluminum gaskets 5 cm

New Opposed Anvil Cell

Studies employ ~50 pressure cells Microbe Pressure Cell Array

Redox Potential  Microbe Pressure Cell Array Pressure 

pH  Microbe Pressure Cell Array Pressure 

Temperature  Microbe Pressure Cell Array Pressure 

Advantages of Pressure Array In situ observations: optical, Raman Significant sample volume Multiple variables: nutrients, redox, pH, temperature, minerals, consortia The anvil cell environment may mimic deep pockets (essentially a closed system).

IV. What Pressure Effects on Biomolecules Might We Study? 1.Pressure induced phase transitions 2.Volumes of reactions 3.Activation volumes 4.Pressure effects on enzymes 5.Diffusion rates and membrane permeability

1. Pressure Induced Phase Transitions Pressure induces phase transitions in membrane- forming lipid molecules.

Ice VI and VII

2. Volumes of Reaction, ΔV Pressure may suppress reactions if ΔV > 0.

2. Volumes of Reaction, ΔV Polyphosphate cleavage (ATP  ADP) H 4 P 2 O 7 + H 2 O  2H 3 PO 4 ΔV ~ +15 cc/mol for P < 1 GPa and T < 200°C

2. Volumes of Reaction, ΔV ATP PO 4 + ADP

2. Volumes of Reaction, ΔV Pressure may enhance reactions if ΔV < 0. Methanogenesis: CO 2 + 4H 2  CH 4 + 2H 2 O ΔV ~ -60 cc/mol for P < 1 GPa and T < 200°C

2. Volumes of Reaction, ΔV Methanogenesis may be enhanced by P Methanococcus jannaschii Methanopyrus kandleri Methanothermobacter thermoautotrophicum thermoautotrophicum

3. Activation Volumes Activation volume is defined as the difference between the partial molar volumes of the initial state and the transition state: P

3. Activation Volumes If activation volume is negative, then reaction rates increase with P. Bond formation; condensation Charge concentration Fe 2+ Fe3+

3. Activation Volumes If activation volume is positive, then reaction rates decrease with P. Unfolding; racemization L-ASP D-ASP

4. Pressure Effects on Activity and Denaturation of Enzymes Fructose diphosphatase (FDPase) at 150 MPa (fish) Hochachka et al. (1970) Marine Biology 7, Hochachka et al. (1970) Marine Biology 7, Lactic dehydrogenase deactivation (rabbits) Schmid et al. (1975) Biophys. Chem. 3, Schmid et al. (1975) Biophys. Chem. 3, Pyrophosphatase activity (Bacillus) Morita & Mathemeier (1964) J. Bacteriology 88, Morita & Mathemeier (1964) J. Bacteriology 88, Protease activity (Methanococcus) Michels & Clark (1997) Appl. Environ. Microbiology 63, Michels & Clark (1997) Appl. Environ. Microbiology 63,

4. Pressure Effects on Microbial Enzymes Use pressure cell array to: Identify and analyze stress proteins Identify and analyze stress proteins Measure metabolic rates Measure metabolic rates Survey gene expression (using mRNA) Survey gene expression (using mRNA)

5. Diffusion rates and Membrane Permeability Pressure decreases diffusion rates and membrane permeability. Pressure increases relative diffusion rate of hydrogen Hydrogen may be an optimal energy source for long-term survival of microbes at high P. [Morita (2000) Microbial Ecology 38: ]

Conclusions Pressure has the potential to slow microbial metabolism by several mechanisms: Pressure has the potential to slow microbial metabolism by several mechanisms: Positive volumes of reactions. Positive activation volumes of reactions Reduced enzyme activites Reduced diffusion rates Reduced membrane permeability More experimental studies are needed.

With thanks to: NASA Astrobiology Institute National Science Foundation Carnegie Institution of Washington