Thermostability of model protocell membranes
Sheref S. Mansy* and Jack W. Szostak†
Howard Hughes Medical Institute, Department of Molecular Biology and Center for Computational and Integrative Biology, Massachusetts General
Hospital, Boston, MA 02114
Edited by Gerald F. Joyce, The Scripps Research Institute, La Jolla, CA, and approved July 8, 2008 (received for review May 26, 2008)
W
e have recently described a laboratory model of a simple
protocell that is useful for assessing the interactions and
compatibility of the protocell components. We found that protocell membranes composed of fatty acids and related molecules
are reasonably permeable to nucleoside phosphorimidazolides
and that efficient template directed copying reactions can take
place in the vesicle interior after the addition of external
activated nucleotides (1). These observations provide strong
support for the plausibility of the heterotrophic protocell model
but immediately bring to mind several additional questions. Most
important, if a genetic polymer is copied inside membrane
vesicles, how could the strands of the double-stranded product
be separated? The possibility of thermal strand separation, as in
PCR, has seemed problematic in view of the presumed thermal
instability of fatty-acid-based vesicles (2, 3). A second question
is whether there might be environmental conditions that could
facilitate nucleotide uptake, allowing more efficient replication
or perhaps the utilization of more highly charged substrates such
as nonactivated nucleotides, nucleoside polyphosphates, or short
oligonucleotides (3). Again, high temperatures would seem likely
to help, but this possibility has not been explored because of the
assumption that such conditions would disrupt vesicle integrity
and lead to the release of contents, including genetic materials,
to the environment. The assumption of thermal instability is
based on the instability of fatty-acid vesicles under several
environmental conditions that do not affect phospholipid vesicles. For example, the critical aggregate concentrations for fatty
acids are much higher than for phospholipids (4), and dilution of
vesicles below this concentration leads to vesicle dissolution.
Also, divalent cations such as Mg2⫹ and Ca2⫹ are very destabilizing to fatty-acid vesicles, because the salts of fatty acids tend
to crystallize out of solution (5, 6). Furthermore, vesicles composed solely of fatty acids are only stable within a fairly narrow
pH range (4), although stability to high pH can be conferred by
admixture with fatty alcohols and fatty-acid glycerol esters (7).
However, as we show here, these environmental sensitivities do
not extend to temperature, and certain fatty-acid-based vesicles
www.pnas.org兾cgi兾doi兾10.1073兾pnas.0805086105
Results
Retention of DNA Oligonucleotides at High Temperatures. We ini-
tially examined the thermal stability of 2:1 myristoleic acid
(MA)/monomyristolein (GMM) vesicles, because this composition leads to vesicles that tolerate a wide range of salt and pH
conditions, including the presence of up to 4 mM Mg2⫹ (5, 6).
We tested vesicle stability by encapsulating a fluorescein-labeled
10-mer oligodeoxynucleotide (dA10), removing unencapsulated
DNA by size-exclusion chromatography (SEC), and then incubating aliquots of the purified vesicles at different temperatures
for 1 h. The fraction of the oligonucleotide that was released
from the vesicles during the high-temperature incubation was
determined by a second round of size-exclusion chromatography, with free and encapsulated DNA measured by fluorimetry.
Surprisingly, 2:1 MA/GMM vesicles remained completely stable
to 100°C, with no detectable release of the encapsulated oligonucleotide (Fig. 1) or change in vesicle size (measured by
dynamic light scattering). However, longer high-temperature
incubation times did result in significant leakage (⬇20% released after 10 h at 100°C).
To test whether this temperature stability is a general feature
of vesicles composed of single-chain amphiphiles or is a unique
characteristic of 2:1 MA/GMM vesicles, we examined vesicles
made with a variety of amphiphiles and amphiphile mixtures by
using the same oligodeoxynucleotide retention assay (Fig. 1). We
examined four pure fatty acids at pH 8.5, which is approximately
the pH at which half of the fatty acid is ionized and half is
protonated, and which corresponds to the pH of maximum
stability because every protonated carboxylate can act as a
hydrogen bond donor to an adjacent ionized carboxylate (4, 8).
Pure myristoleic acid (C14:1) vesicles released small amounts of
DNA after 1 h at 50°C, with increasing amounts released at
higher temperatures (⬇10–20% released after 1 h at 60–80°C).
Palmitoleic acid (C16:1) and oleic acid (C18:1) vesicles were
completely stable to 90°C, but did show 30–35% leakage of
entrapped DNA after 1 h at 100°C (Fig. 1 A). Thus, increasing
chain length leads to increased thermal stability of the bilayer
membrane, consistent with membrane stabilization through the
entropic effect of water release as the hydrophobic acyl chains
are buried in the membrane (9). We also examined linoleic acid
(C18:2) vesicles; this lipid leads to more fluid membranes with
increased permeability to nucleotides at low temperatures (1).
This C18:2 fatty acid behaved similarly to the C18:1 oleic acid,
with linoleic acid vesicles being completely stable to 90°C but
Author contributions: S.S.M. and J.W.S. designed research; S.S.M. performed research;
S.S.M. and J.W.S. analyzed data; and S.S.M. and J.W.S. wrote the article.
The authors declare no conflict of interest.
Freely available online through the PNAS open access option.
*Present address: Department of Chemistry and Biochemistry, University of Denver, Denver, CO 80208.
†To whom correpondence should be addressed. E-mail: szostak@molbio.mgh.harvard.edu.
© 2008 by The National Academy of Sciences of the USA
PNAS 兩 September 9, 2008 兩 vol. 105 兩 no. 36 兩 13351–13355
CHEMISTRY
origin of life 兩 RNA world 兩 synthetic biology 兩 vesicle 兩 prebiotic
are remarkably thermostable. This observation extends the
range of environments that could be tolerated by early cells and
opens up ways in which thermal fluctuations could be used to
advantage by primitive cells.
BIOPHYSICS
The earliest cells may have consisted of a self-replicating genetic
polymer encapsulated within a self-replicating membrane vesicle.
Here, we show that vesicles composed of simple single-chain
amphiphiles such as fatty acids, fatty alcohols, and fatty-acid
glycerol esters are extremely thermostable and retain internal RNA
and DNA oligonucleotides at temperatures ranging from 0°C to
100°C. The strands of encapsulated double-stranded DNA can be
separated by denaturation at high temperature while being retained within vesicles, implying that strand separation in primitive
protocells could have been mediated by thermal fluctuations
without the loss of genetic material from the protocell. At elevated
temperatures, complex charged molecules such as nucleotides
cross fatty-acid-based membranes very rapidly, suggesting that
high temperature excursions may have facilitated nutrient uptake
before the evolution of advanced membrane transporters. The
thermostability of these membranes is consistent with the spontaneous replication of encapsulated nucleic acids by the alternation
of template-copying chemistry at low temperature with strandseparation and nutrient uptake at high temperature.
Fig. 1. Thermostability of model protocell membranes. The leakage of a fluorescein-labeled dA10 oligonucleotide from vesicles of the indicated composition
was monitored as a function of time. (A) Influence of the acyl chain on vesicle stability. {, 2:1 decanoic acid/decanol; F, MA; Œ, palmitoleic acid; }, oleic acid;
■, linoleic acid; 䊐, 2:1 MA/farnesol. (B) Influence of the head group on C14:1 vesicle stability. ■, MA; Œ, 2:1 MA/MA-OH; F, 2:1 MA/GMM. Identical results were
given for 2:1 palmitoleic acid/monopalmitolein and 2:1 oleic acid/monoolein as for 2:1 MA/GMM (C) Time-dependent leakage from 2:1 MA/GMM vesicles at
100°C. (D) Influence of the head group on C10:0 vesicle stability. ■, 2:1 decanoic acid/decanol; F, 4:1:1 decanoic acid/decanol/monocaprin. (E) Time-dependent
leakage from 4:1:1 decanoic acid/decanol/monocaprin model prebiotic vesicles at 100°C. Solution conditions were 0.2 M sodium bicine, pH 8.5.
exhibiting ⬇20% release of encapsulated DNA after 1 h at
100°C.
We then examined the effect on vesicle stability of a series of
additives to pure MA. As noted above, MA/GMM (2:1) vesicles
are stable during prolonged incubation at 100°C, presumably
because of the ability of the glycerol headgroup to provide two
hydrogen bond donors that can interact with the ionized carboxylates of MA. Consistent with this argument, myristoleyl
alcohol (MA-OH), which can provide one hydrogen bond donor
per molecule, also stabilizes MA vesicles, but less effectively than
GMM. To determine whether the thermostability of vesicles
composed of longer-chain fatty acids could be similarly improved, we examined mixtures of palmitoleic acid and oleic acid
with their corresponding glycerol monoester derivatives. As
expected, in both cases the addition of the glycerol monoester
lipid conferred stability at 100°C, and no leakage of encapsulated
DNA was observed (Fig. 1B). Thus, vesicle thermostability can
be enhanced either by strengthening head group interactions
(e.g., adding GMM or M-OH to MA) or acyl chain interactions
(e.g., increasing chain length from 14 to 16 to 18 carbons). In
contrast, the highly branched isoprenoid alcohol farnesol decreased vesicle stability, presumably by weakening acyl chain
interactions (Fig. 1 A).
We examined the stability of vesicles composed of short-chain
(C10) saturated amphiphiles (Fig. 1D) because these molecules
are more prebiotically plausible than longer-chain unsaturated
amphiphiles. Pure capric acid (C10:0, decanoic acid) vesicles, as
previously reported (4) are only stable at ⱖ50 mM total amphiphile concentration; these vesicles were too unstable to purify by
size-exclusion chromatography (10), and therefore, we were
unable to measure their ability to retain dA10 at elevated
temperatures. However, synthesis by modified Fischer–Tropsch
Type (FTT) chemistry is likely to yield a mixture of hydrocarbons, alcohols, aldehydes, and acids (11, 12), and glycerol esters
of fatty acids could form in a typical ‘‘drying lagoon’’ scenario
(13). Therefore, we examined mixtures of capric acid with some
of these related compounds (Fig. 1D). Vesicles of 2:1 capric
13352 兩 www.pnas.org兾cgi兾doi兾10.1073兾pnas.0805086105
acid/decanol were somewhat more thermostable, but started to
leak encapsulated oligonucleotide at 50–60°C. Vesicles of 2:1
capric acid/monocaprin could be observed by microscopy and
were capable of retaining an entrapped oligonucleotide, as
evidenced by dialysis and microscopy, but were not stable
enough to survive gel filtration chromatography and gradually
crystallized overnight at room temperature. This instability may
reflect the large ratio of head group size to acyl chain length for
monocaprin. To decrease the average head group size, we
explored ternary mixtures of capric acid with decanol and
monocaprin. Interestingly, these exhibited significantly increased thermostability and retained oligonucleotides for 1 h at
60–70°C and could tolerate shorter periods of high temperatures
up to 100°C for 1 min with no detectable loss of encapsulated
oligonucleotide (Fig. 1E). These experiments show that amphiphile mixtures of the kind that may have been present on the
early earth could encapsulate nucleic acids and retain these at
least for brief periods at high temperature.
We wondered whether observed temperature stability extends
to multiple thermocycles or whether rapid and large changes in
temperature result in vesicle disruption. To answer this question,
we subjected MA/GMM (2:1) vesicles to 20 cycles of 2 min at
20°C and 2 min at 90°C, and we quantified the loss of entrapped
oligonucleotide. After 20 cycles, no loss of nucleic acid was
observed. We then examined the response of prebiotic-model
vesicles [decanoic acid (DA)/decanol (DOH)/glycerol monoester
of decanoic acid (GMD)::4:1:1] to a similar thermocycling
regime (20 cycles of 30 s at 25°C and 30 s at 90°C). In this case,
10–20% of the labeled DNA contents did leak out over 20 cycles,
corresponding to a loss of 0.5–1.0% of contents per cycle. The
stability of vesicles to multiple thermocycles is an important
characteristic because it demonstrates that vesicles composed of
simple single-chain amphiphiles are capable of surviving environments such as hydrothermal vents and hot springs that are
candidates for sites of early evolution (14).
DNA Strand Separation within Vesicles. We used an oligonucleotide
FRET pair strategy to demonstrate that vesicle thermostability
Mansy and Szostak
Fig. 2. Intravesicular DNA strand melting. (A) Schematic representation of
the experimental setup. Black bars represent DNA molecules either modified
with a fluorophore (D) or quencher (Q). White bars represent unlabeled
strands of DNA. (B) Increase in fluorescence arising from intravesicular DNA
strand melting and annealing. C, control; A, 2:1 MA/GMM; B, 4:1:1 decanoic
acid/decanol/monocaprin; S, solution reaction (that is, not inside vesicles). The
control reaction was of the same composition but not subjected to a thermocycle.
ously shown that activated nucleotides can spontaneously diffuse
across the fatty-acid-based bilayer membranes, so that nucleotides added to the outside can enter vesicles and take part in
template-directed primer-extension reactions on the inside of
the vesicle (1). Nucleotide permeation appears to operate via a
concerted flipping of an amphiphile-solute complex as opposed
to packing defects arising from gel to liquid phase transitions, as
seen for dimyristoyl phosphatidylcholine membranes (15). When
we realized that these vesicles are stable to elevated temperatures, we wondered whether nucleotide permeability would be
significantly enhanced at higher temperatures. By encapsulating
radiolabeled nucleotides, incubating at high temperatures, followed by SEC to resolve retained and leaked nucleotides, we
were able to observe rapid permeation of activated nucleotides,
with uridine-5⬘-phosphorimidazolide equilibrating across 2:1
MA/GMM membranes within 30 s at 90°C. Because our previous
low-temperature data demonstrated that the permeability of
nonactivated nucleotide monophosphates was significantly
slower than activated nucleotides (1), we sought to determine
whether high temperatures would also increase the permeability
of unactivated nucleoside monophosphates. Unactivated NMPs
are much less permeable than activated NMPs because the
phosphate bears two negative charges instead of one. We
observed that the permeability of the more polar nonactivated
nucleoside monophosphates dramatically increased, with release
of encapsulated nucleotides from 100-nm MA/GMM vesicles
reaching completion within 10 min for AMP, GMP, CMP, UMP,
and deoxyadenosine-5⬘-monophosphate (dAMP) (Fig. 3A). Under the same solution conditions but at 23°C, ⬍10% of nucleMansy and Szostak
Fig. 3. High-temperature nucleotide permeability. (A) Nucleotide monophosphate permeability of 2:1 MA/GMM vesicles at 90°C. , AMP; ƒ, AMP ⫹
MgCl2, F, CMP; E, CMP ⫹ MgCl2, }, GMP; {, GMP ⫹ MgCl2, ■, UMP; 䊐, UMP ⫹
MgCl2. (B) Influence of 5⬘ phosphates on 2:1 MA/GMM vesicle permeability at
90°C. F, AMP; E, AMP ⫹ MgCl2; Œ, ADP; ‚, ADP ⫹ MgCl2; ■, ATP; 䊐, ATP ⫹ MgCl2.
(C) Oligomer permeability of 2:1 MA/GMM vesicles after a 1-h incubation at each
indicated temperature. ■, NAD; F, AAA; E, AAAA.
oside monophosphates crossed the membrane over a 24-h period
(1). We further probed the influence of charge by measuring the
permeation of ADP and ATP (Fig. 3B). In the absence of Mg2⫹,
ADP crossed the membrane more slowly than AMP (⬇20 min
for complete equilibration of ADP vs. ⬍10 min for AMP);
however, in the presence of Mg2⫹, ADP permeated more rapidly
than AMP (complete equilibration in ⬍3 min), consistent with
the higher affinity of ADP for Mg2⫹ (16) and consistent with
previously observed trends at 23°C (1). ATP permeation was
much slower (⬎1 h for completion) and could not be fit to a
single exponential curve. Simple prebiotic model membranes are
clearly more robust than previously appreciated, allowing for
conditions, such as elevated temperatures, that facilitate the
uptake of critical nutrients without the loss of larger entrapped
material such as oligonucleotides.
Although the vesicle stability and nucleotide permeability
characteristics of these membrane compositions are clearly
compatible with PCR, we were unable to successfully reconstitute PCR within fatty-acid vesicles, most likely due to the strong
inhibition of DNA polymerases by even low concentrations of
fatty acids (17). PCR within phospholipid vesicles has been
previously documented, but because of the impermeability of the
PNAS 兩 September 9, 2008 兩 vol. 105 兩 no. 36 兩 13353
CHEMISTRY
Nucleotide Permeability at Elevated Temperatures. We have previ-
BIOPHYSICS
can be exploited for DNA strand separation and reannealing
within vesicles. Complementary 19-mer oligodeoxynucleotides
that were labeled with a fluorophore and a quencher at their 5⬘
and 3⬘ ends, respectively, were annealed and mixed with an
excess of unlabeled oligonucleotide duplex of exactly the same
sequence (Fig. 2). Heating above the Tm of the dsDNA (75°C)
leads to strand separation, and subsequent cooling allowed
random reannealing of labeled and unlabeled oligonucletides,
thus yielding an increase in fluorescence. This assay was applied
to both 2:1 MA/GMM and 4:1:1 capric acid/decanol/monocaprin
vesicles with a 1-min incubation at 90°C, followed by cooling to
20°C for reannealing. After size-exclusion chromatography to
ensure that only encapsulated DNA was monitored, both vesicle
compositions gave rise to the increased fluorescence signal that
is diagnostic of strand separation and reannealing. The measured
fluorescence increase was similar to control reactions in solution
and consistent with complete strand melting and reannealing as
a result of thermocycling within vesicles.
membrane, the nucleotides had to be encapsulated during vesicle
formation rather than delivered across the membrane (18).
Permeability of Oligonucleotides. The permeation of mononucleo-
side diphosphates and triphosphates, but not a 10-mer oligonucleotide, suggested that short oligonucleotides might cross the
membrane at elevated temperatures. Therefore, we measured
the retention of a series of oligomers within 100-nm MA/GMM
(2:1) vesicles at 90°C. In the absence of Mg2⫹, dinucleoside
diphosphates (NppN) required 4 min for 50% leakage from the
vesicles, whereas trinucleotides (pNpNpN) leaked out more
slowly, with 50% loss after 37 min. Tetranucleotides were
completely retained after 1 h at 90°C (Fig. 3C). Thus, protocell
replication schemes that invoke the sequential templated ligation
of oligonucleotide substrates are only feasible for dinucleotides
and trinucleotides, assuming that the substrates are taken up
from the external environment. Alternatively, the intracellular
generation of substrate oligonucleotides of length ⱖ4 could be
used to generate a pool of trapped substrates for replication,
while entrapped molecules smaller than a tetramer would be
rapidly lost to the environment at 90°C.
Discussion
The high thermal stability of the model protocell membranes
that we have studied has significant implications for the origin of
cellular life. At the most basic level, our results suggest that even
very primitive, self-assembled protocell structures could survive
in environments with large and/or frequent temperature fluctuations. Thus, consideration of appropriate environments for
the origin of the first cells need not be limited to sheltered
subsurface locales, but can also reasonably include surface and
near-surface locations subject to diurnal temperature variations,
as well as locations near heat sources such as hydrothermal vents
and hot springs. Perhaps more interesting than the simple ability
of early cells to tolerate temperature fluctuations is the possibility that primitive cells could take advantage of thermal cycling
to facilitate both strand separation of replicated genomic templates and the rapid uptake of nutrients during high-temperature
excursions. For example, one could imagine a primitive ‘‘cell
cycle,’’ in which replication of the genetic material and growth
of the vesicle compartment proceed at low to moderate temperatures, interrupted by high-temperature interludes that lead
to strand separation and the influx of additional nucleotides. Cell
division, perhaps triggered by environmental shear forces, would
lead to random assortment of genetic molecules into daughter
cells.
Diurnal temperature fluctuations are frequently invoked in
prebiotic scenarios as a means of cyclic concentration by evaporative drying followed by redissolution, or as a means of driving
chemical transformations within evaporated materials. Such
temperature fluctuations could also drive periodic strand separation and nutrient uptake in vesicles, but the length of the
diurnal cycle, even on the early earth, would lead to significant
leakage of genetic polymers from primitive cells unless the cell
membranes were composed of fairly long-chain fatty acids.
Another attractive possibility for an environment that would
subject primitive cells to large thermal fluctuations is provided
by the possibility of convection cells near or within surface hot
springs or hydrothermal vents. Rayleigh–Bernard convection
cells have been shown, in the laboratory, to allow for the rapid
cycling of DNA molecules between moderate and high temperatures, leading to amplification by PCR (19, 20). On the early
earth, such convection cells might subject an adjacent fluid
reservoir containing a population of replicating protocells to
brief periods of high temperature, sufficient for strand separation and enhanced nutrient uptake separated by long and
random interludes at lower temperatures.
13354 兩 www.pnas.org兾cgi兾doi兾10.1073兾pnas.0805086105
A third significant and surprising outcome of our experiments
is that mixtures of amphiphiles seem to form membranes with
more desirable characteristics than membranes composed of
single, pure amphiphiles. Previous studies have shown that the
addition of fatty alcohols and fatty-acid glycerol esters to pure
fatty acids lead to membranes that are more tolerant to the
presence of divalent cations (5), and which show increased
permeability (1) to sugars and nucleotides. Our current work
shows that such mixtures form membranes with dramatically
enhanced thermostability, compared with pure fatty-acid membranes. Because prebiotic chemical reactions undoubtedly generated complex mixtures of lipids, rather than a single lipid
species, it is plausible that vesicles assembled from such prebiotic
mixtures might have had greater thermostability, ion tolerance,
and permeability than more homogeneous laboratory model
vesicles. This behavior is in striking contrast to the situation with
genetic polymers, where the availability of a relatively homogeneous set of initial nucleotides is generally regarded as essential
to the synthesis of useful oligonucleotides. For example, stereochemical purity is important for RNA replication, as the
presence of contaminating incorrect enantiomers leads to the
strong inhibition of further polymerization (21).
Materials and Methods
Materials. Fatty acids, fatty alcohols, and the glycerol monoesters of fatty acids
were obtained from Nu Chek Prep. All other chemicals were obtained from
Sigma–Aldrich.
Vesicle Preparation. Fatty-acid vesicles were prepared by oil dispersion in
buffered solutions as previously described (22, 23). For vesicles composed of
mixtures of amphiphiles, the oils were mixed before dispersion in aqueous
solution. All vesicle preparations were extruded 11 times through 100-nm
pore-size polycarbonate filters with an Avanti miniextruder (Avanti Polar
Lipids). For the encapsulation of molecules, amphiphiles were resuspended in
the presence of the encapsulant. Separation of entrapped and unencapsulated material was by gel filtration with Sepharose 4B resin (Sigma–Aldrich) in
which the running buffer contained the same amphiphile composition as the
vesicles at a concentration above their critical aggregate concentration. Vesicle size was measured by dynamic light scattering with a PDDLS/CoolBatch
90T (Precision Detectors).
Nucleotide Permeability. Nucleotide permeability measurements were made
in 0.2 M sodium bicine, pH 8.5. Radioactive nucleotides (0.1 mM) were encapsulated, and the vesicles were purified by gel filtration (Sepharose 4B). Vesicles
were incubated at different temperatures in a Bio-Rad DNA Engine Peltier
thermal cycler. Samples were then loaded on a gel filtration column, collected
with a Gilson FC 203B fraction collector, and analyzed by scintillation counting
with UniverSol scintillation fluid (MP biomedicals) on a Beckman Coulter LS
6500 multipurpose scintillation counter. Isotopes were either 14C or 3H and
were obtained from Moravek Biochemicals and Radiochemicals.
Vesicle Stability and Oligonucleotide Permeability. The assay was as described
for nucleotide permeability except that oligonucleotides were used in place of
mononucleotides. Oligonucleotide sequences were poly(A), except for the
dimer, and were either synthesized at the Massachusetts General Hospital
DNA core facility or the Yale University Keck facility (New Haven, CT). The
10-mer had a covalently attached 5⬘-fluorescein. The dimer was 3H-labeled
NAD (Moravek Biochemicals and Radiochemicals). Trimer and tetramer oligonucleotides were 5⬘-labeled by using 32P-␥-ATP and T4 polynucleotide kinase
(New England Biolabs). Fluorescence was measured with a SpectraMAX GeminiEM fluorescence plate reader (Molecular Devices).
Strand Melting Assay. Fluorescently labeled oligodeoxynucleotides were obtained from Integrated DNA Technologies; 5⬘-ATGCGCCCGGCCTAGGGCC-3⬘
was synthesized with a 5⬘ tetrachlorofluorescein modification, and 5⬘GGCCCTAGGCCGGGCGCAT-3⬘ was synthesized with a 3⬘ black hole
quencher-1 (BHQ-1) modification. MA/GMM (2:1) samples were incubated at
20°C for 2 min, 90°C for 1 min, and 20°C for 2 min before measurement on
SpectraMAX GeminiEM fluorescence plate reader (Molecular Devices) with
excitation and emission at 518 and 539 nm, respectively.
Mansy and Szostak
by NASA Exobiology Program Grant EXB02– 0031-0018. J.W.S. is an Investigator of the Howard Hughes Medical Institute. S.S.M. was supported in part by
the National Institutes of Health Award F32 GM07450601.
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CHEMISTRY
ACKNOWLEDGMENTS. We thank J. P. Schrum, R. J. Bruckner, M. M. Hanczyc,
B. Seelig, I. A. Chen, S. Tobé, T. F. Zhu, Q. Dufton, J. Iwasa, F. P. Seebeck, A.
Ricardo, A. J. Bell, and M. Sam for helpful discussions. This work was supported
Mansy and Szostak
PNAS 兩 September 9, 2008 兩 vol. 105 兩 no. 36 兩 13355