Science - USA - 03.12.2021

requires an alternative pathway that is med-
iated by the 3′exonuclease activities of Pold,
which removes nucleotides from the 3′end of
an upstream Okazaki fragment, generating a
gap for the unprocessed 5′flap to reanneal for
ligation ( 16 , 23 ). Restrictive temperature stress
activates Dun1 signaling and stimulates de
novo production of deoxyribonucleotides, which
in turn inhibits the 3′exonuclease activity, but
not the flap nuclease activity of Pold, and in-
duces other DNA damage responses. These
molecular changes push OFM toward trans-
formation of an unprocessed 5′flap into a 3′
flap, either through flap equilibration ( 24 ) or
through the actions of helicases such as Sgs1 or
Pif1, leading to a secondary structure that may
result in alternative duplications, including
Pold-ITD, in revertant strains. In the rever-
tants, Poldmutations limit DNA displacement,
thus suppressing 5′flap formation or allowing
moretimeforDna2orExo1toactonthe5′
flap and bypass the requirement for Rad27
(Fig. 4G).

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ACKNOWLEDGMENTS
We thank R. Kolodner for the yeast strains RDKY2672, RDKY2608,
and RDKY2669; P. M. J. Burgers for the plasmids pBL335 (GST-
Pol3), pBL338 (GAL1-Pol31), pBL340 (GAL10-Pol32), and pBL341
(Pol31/Pol32); L. Prakash and S. Prakash for the protease-deficient
yeast strain YRP654 and the plasmids pBJ1445 (Flag-Pol3) and
pBJ1524 (GST-Pol31/Pol32) to express the yeast recombinant Pold

complex (Pol3, Pol31, and Pol32); W.-D. Heyer for the anti-Dun1

antibody; and M. S. Wold for purified recombinant yeast replication

protein A (RPA) complex. We thank H. Lou’s laboratory members

and H. Dai, D. Duenas, and M. E. Budd for technical assistance in

mouse and yeast genetic experiments and stimulating discussions.

We thank K. Walker and S. Wilkinson for critical reading and editing

of the manuscript.Funding:This work was supported by NIH

grants R50 CA211397 to L.Z. and R01 CA073764 and R01

CA085344 to B.S. Research reported in this publication includes

work performed by City of Hope shared resources supported by

the National Cancer Institute of the NIH under award number P30

CA033572.Author contributions:H.S., Z.L., A.S., Y.Z., and M.Z.

conducted yeast genetic and biochemical experiments. E.Z., J.W.,

X.W., Z.H., and Z.G. conducted RNA sequencing (RNA-seq), WES,

and WGS and performed data analysis. J.L.C. designed yeast

genetic experiments and conducted data analysis. L.Z. conducted

biochemical experiments, RNA-seq, and WGS data analysis;

designed and coordinated most of the experiments; and wrote the

first draft of the manuscript. B.S. supervised the entire project;

designed and coordinated most of the experiments; and provided

input into and finalized the manuscript.Competing interests:The

authors declare no conflicts of interest in this study.Data and

materials availability:All data are available in the manuscript or

the supplementary materials. Gene Expression Omnibus accession

numbers for the mouse and yeast genomics datasets are

GSE181154 and GSE178876, respectively.

SUPPLEMENTARY MATERIALS

science.org/doi/10.1126/science.abj1013

Materials and Methods

Supplementary Text

Figs. S1 to S20

Tables S1 to S6

References ( 25 Ð 51 )

MDAR Reproducibility Checklist

20 April 2021; accepted 14 October 2021

10.1126/science.abj1013

ORGANIC CHEMISTRY

A biomimetic SH2 cross-coupling mechanism for

quaternary sp

3

-carbon formation

Wei Liu^1 †, Marissa N. Lavagnino^1 †, Colin A. Gould^1 , Jesús Alcázar^2 , David W. C. MacMillan^1 *

Bimolecular homolytic substitution (SH2) is an open-shell mechanism that is implicated across

a host of biochemical alkylation pathways. Surprisingly, however, this radical substitution

manifold has not been generally deployed as a design element in synthetic C–C bond formation. We

found that the SH2 mechanism can be leveraged to enable a biomimetic sp^3 -sp^3 cross-coupling

platform that furnishes quaternary sp^3 -carbon centers, a long-standing challenge in organic

molecule construction. This heteroselective radical-radical coupling uses the capacity of iron

porphyrin to readily distinguish between the SH2 bond-forming roles of open-shell primary and

tertiary carbons, combined with photocatalysis to generate both radical classes simultaneously

from widely abundant functional groups. Mechanistic studies confirm the intermediacy of a primary

alkyl–Fe(III) species prior to coupling and provide evidence for the SH2 displacement pathway

in the critical quaternary sp^3 -carbon bond formation step.

O

ver the past five decades, transition

metal–catalyzed cross-coupling has com-

prehensively transformed the landscape

of molecule construction in the applied

sciences, especially with respect to phar-

maceuticals, agrochemicals, and functional

materials ( 1 , 2 ). In particular, the combination

of three mechanistic steps—oxidative addition,

transmetalation, and reductive elimination—

has served as a robust catalytic paradigm for

C–C bond formation, enabling a highly mod-

ular yet general approach to fragment cou-

pling (Fig. 1A). Although this paradigm has

proven to be exceptionally successful for

forging C(sp^2 )–C(sp^2 ) bonds, it is important to

recognize that each of these three elementary

steps is less efficient when transition metals

engage with secondary or tertiary alkyl frag-

ments, limiting the development of a C(sp^3 )–

C(sp^3 ) cross-coupling platform of broad util-

ity ( 3 – 6 ).

It is intriguing to consider that enzymatic

formation of C(sp^3 )–C(sp^3 ) bonds proceeds by

fundamentally different open-shell pathways

to achieve pivotal alkylation reactions ( 7 , 8 ).

As one canonical example, methylcobalamin

systems serve as nature’s“free radical carrier”

by stabilizing otherwise highly reactive methyl

radicals ( 9 , 10 ). As such, in cobalamin-dependent

radicalS-adenosylmethionine (SAM) meth-

yltransferases, transiently generated carbon-

centered radicals can react with these alkyl-

cobalt complexes via bimolecular homolytic

substitution (SH2) (Fig. 1B) ( 11 ). Although

cobalamin provides critical stabilization to

the reactive methyl radical, the methyl-cobalt

bond remains notably weak (bond dissocia-

tion energy = ~37 kcal/mol), which underpins

the kinetic preference for the SH2 mechanism

and heteroselective carbon-carbon bond for-

mation ( 12 ). Elegant biosynthetic studies have

shown that the rates of such enzymatic SH 2

reactions are extremely fast (~ 10^8 s–^1 ) and

enable the formation of sterically congested

1258 3 DECEMBER 2021•VOL 374 ISSUE 6572 science.orgSCIENCE

(^1) Merck Center for Catalysis at Princeton University,
Princeton, NJ 08544, USA.^2 Discovery Chemistry, Janssen
Research and Development, Janssen-Cilag S.A., C/Jarama
75A, Toledo 45007, Spain.
*Corresponding author. Email: [email protected]
†These authors contributed equally to this work.
RESEARCH | REPORTS