ARTICLE

Received 23 Sep 2014 | Accepted 18 Nov 2014 | Published 20 Jan 2015

Periploside A is a pregnane hexasaccharide identied from the Chinese medicinal plant Periploca sepium, which features a unique seven-membered formyl acetal bridged orthoester (FABO) motif and potent immunosuppressive activities. Here, we show the synthesis of this molecule in a total of 76 steps with the longest linear sequence of 29 steps and 9.2% overall yield. The FABO motif is constructed via a combination of Sinas and Crichs protocol for the formation of orthoester and acetal glycosides, respectively. The 2-deoxy-b-glycosidic linkages are assembled stereoselectively with judicious choice of the glycosylation methods. The epimer at the spiro-quaternary carbon in the FABO motif has also been elaborated in a stereo-controlled manner. This epimer, as well as the synthetic analogues bearing the FABO motif, retain largely the inhibitory activities of periploside A against the proliferation of T-lymphocyte, indicating the importance of the chemical connection of the FABO motif to their immunosuppressive activity.

DOI: 10.1038/ncomms6879 OPEN

Total synthesis of periploside A, a unique pregnane hexasaccharide with potent immunosuppressive effects

Xiaheng Zhang1, Yu Zhou2, Jianping Zuo2 & Biao Yu1

1 State Key Laboratory of Bioorganic and Natural Products Chemistry, Shanghai Institute of Organic Chemistry, Chinese Academy of Sciences, 345 Lingling Road, Shanghai 200032, China. 2 State Key Laboratory of New Drug Research, Shanghai Institute of Materia Medica, Chinese Academy of Sciences, Shanghai 201203, China. Correspondence and requests for materials should be addressed to B.Y. (email: mailto:[email protected]

Web End [email protected] ).

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Periploside A (or Periplocoside E) is the prototypical member of a group of pregnane glycosides isolated from Periploca sepium and P. forrestii (Asclepiadaceae), which

features a unique seven-membered formyl acetal bridged orthoester (FABO) linkage between two sugar units17. This natural product shows immunosuppressive activities, that is, it inhibits the ConA-induced T cell proliferation as potently as rapamycin and cyclosporin A while showing reasonably low toxicity (IC50 0.64 mM and CC50 10.1 mM)5,6. The

immunosuppressive effects of periploside A has also been found signicant in mice models810, that validates the folkloric reputation of the plant as a traditional Chinese medicine for rheumatoid arthritis11. Such autoimmune diseases as rheumatoid arthritis, multiple sclerosis, systemic lupus erythematosus and Crohns disease, are notoriously malignant and refractory, thus efcacious new immunosuppressant drugs have long been a quest12.

The FABO motif in periplosides, which has been found critical to their activities6, remains ambiguous in both the chemical connection and stereochemistry for over two decades. In 1987, Hikino et al. reported the rst structural assignment of periploside A, in that the connection of the orthoester was proposed on the basis of extensive chemical degradation and spectroscopic analysis1. However, the stereochemistry of the quaternary anomeric carbon was overlooked but drawn in a conguration comprising an unusual a-(1-4)-glycosidic linkage (1a). Shortly afterwards, Itokawa et al.24 suggested a novel peroxy linkage (1b) for periplosides (and named as periplocosides), as misled by a conventional colour reaction of peroxides, although all the analytical data of periplocoside E were found identical to those of the previous periploside A (ref. 3). This peroxide structure was then accepted till 2011 (refs 5,6),

Zhao and coworkers acquired an X-ray diffraction of a single crystal of a periploside congener, conrming the originally assigned FABO connection6. Unfortunately, the stereochemistry of the spiro-quaternary carbon remained incorrect until we examined it carefully during our journey toward the synthesis of periploside A (ref. 7).

Herein, we report the rst total synthesis of periploside A (1), employing total of 76 steps of transformations from glucal, methyl a-D-glucopyranoside and dehydroepiandrosterone, with the longest linear sequence of 29 steps and in 9.2% overall yield. The stereoselective construction of the FABO motif with either the natural or unnatural conguration at the anomeric spiro-quaternary center is achieved via alternative combination of Crichs protocol for acetal glycoside synthesis and Sinas protocol for glycosyl orthoester formation. The 2-deoxy-bglycosidic linkages are synthesized by glycosylation with triuoroacetimidate donors (6/27) equipped with 2-iodide, with digitoxosyl ortho-alkynylbenzoate donor (8) installed with bulky TBDPS group on the remote 3,4-OH, and with cymarosyl orthoalkynylbenzoate donor (2) under the promotion of Ph3PAuOTf/

TTBP. In addition, a preliminary structureactivity relationship of the synthetic periplosides against the proliferation of T-lymphocyte is provided, indicating the importance of the chemical connection of the FABO motif to the activities.

ResultsRetrosynthetic analysis. Given the big size and linear structure of the target molecule, a convergent synthesis was desired13. Thus, periploside A (1) was disconnected into two fragments of similar complexity, that is, tetrasaccharide donor 2 and pregnane FABO disaccharide 3 (Fig. 1). The (1-4)-cymarosyl linkage between

HO

MeO

O

O

O

O

O

O

O

O

O

O

O

OO

O

O

O

20

O O

O

O

or

O

Me

O

OMe

OMe

OMe

O

OH

O

O

H

17

Periploside A (1)

1a 1b

H H

HO

3

O

O

HO

MeO

O

O

O

CAO

MeO

OAc

O

O

O

O

O

O

O

O

O

O

+

OH

OMe

OMe

OMe

2 3

O

TBSO

HO

Br

CAO

MeO

OAc

O

O

O

O

OH

O

O

HO OMP

O

O

O

O CF3

NPh

+

O

BzO

MeO

+

O

O

I

OMe

OMe

OMe

4 6 7

5

TBSO

O

Br

TBDPSO O

TBDPSO O

8 10 11

O

SePh

O

Br

RO MeO

O

O

HO O

O

BzO

MeO

SePh

OCH2SPh

AcO

+ HO

OMP

OMP

I

9

I

Figure 1 | Periploside A 1 and the retrosynthetic analysis. Shadowed in pale blue are the FABO motifs that have been previously assigned; highlighted in red are leaving groups in donors and in blue are hydroxyl groups in acceptors. Ac, acetyl; CA, chloroacetyl; MP, 4-methoxyphenyl; TBDPS, tertbutyldiphenylsilyl; TBS, tert-butyldimethylsilyl.

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NATURE COMMUNICATIONS | DOI: 10.1038/ncomms6879 ARTICLE

the tetrasaccharide unit and 3 would be difcult to construct in favour of formation of the thermodynamically unfavored banomer1417; the glycosylation protocol with orthoalkynylbenzoates as leaving groups (as in 2) under the catalysis of a gold(I) complex could address this problem, in that substitution via an a-glycosyloxypyrylium or a-triate intermediate might get invoked18. The b-(1-4)-cymarosyl linkages in tetrasaccharide 2, however, could be built stereoselectively under the inuence of a substituent at the axial 3-OH of a digitoxosyl donor, which could subsequently be converted into the required methyl group. In this respect, we had screened carefully during the synthesis of digitoxin and gordonoside F and found gold(I)-catalysed glycosylation with digitoxosyl ortho-cyclopropylethynylbenzoate equipped with two bulky TBDPS groups at 3,4-OH (that is, 8) to be an optimal choice15,17. After furnishing the cymarose trisaccharide 5, its coupling with the terminal digitalose unit could be realized with donor 4, in that the formation of the b-linkage should be secured by participation of the 2-O-acetyl group; and the 4-O-chloroacetyl group was selectively removable afterwards. The p-methoxyphenyl (MP) group was employed throughout (as in 5, 9 and 11) as the anomeric protecting group, which could remain intact before cleavage and subsequently converting the saccharides into donors (for example, 2 and 6).

Uncertainty lies in the synthesis of FABO disaccharide 3. Condensation of 3b-silyloxy-pregnene-17a,20a-diol 7 with disaccharide triuoroacetimidate 6, one of the most reliable type of glycosylation donors19, which was equipped with an equatorial iodide at C2 (ref. 20), would lead to the desired C20-O-bglycoside 3 in a regio- and stereo- selective manner. However, few clues occur in the literatures, which could lead to the construction of a disaccharide precursor consisting of the FABO linkage. The most promising approach turned out to be a combination of Crichs protocol to form the formyl acetal glycosidic linkage

(from a thiomethyl glycoside donor such as 10; ref. 21) and Sinas protocol to synthesize the anomeric orthoester via a ketene acetal intermediate (derived from a 2-selenoglycoside such as 9; refs 2224). However, the tolerance of the formyl acetal (in 9) towards the strong conditions required for Sinas oxidation eliminationcyclization sequence and the stereochemistry in the formation of the seven-membered spiro-orthoester were beyond estimation.

Synthesis of tetrasaccharide donor 2. The desired digitalosyl and digtoxosyl ortho-cyclopropylethynylbenzoates 4 and 8 were prepared in a robust manner from D-fucose (13 steps and 37% overall yield) (see Supplementary Methods) and methyl a-D-glucopyranoside (10 steps and 47% overall yield)15, respectively. Subjection of 8 to glycosidation with p-methoxyphenol under optimized conditions (0.1 equivalent (equiv) Ph3PAuNTf2, toluene, 4 molecular sieves (MS), 40 C) led to b-glycoside

12 as the sole anomer in an excellent 95% yield (Fig. 2). Removal of the 3,4-di-O-TBDPS group followed by selective acetylation of the axial 3-OH via orthoester formation/hydrolysis provided glycoside 13 bearing a free 4-OH (92%, two steps)25. Similar transformations were then applied to extend monosaccharide 13 to trisaccharide 17, in that the glycosidation of 8 with monosaccharide acceptor 13 and disaccharide acceptor 15 led to the corresponding coupled 2-deoxy-b-saccharides nearly quantitatively. Trisaccharide 300,400-diol 17 was then subjected to a tin-mediated selective benzylation on the equatorial 400-OH (ref. 26); cleavage and scramble of the acetyl groups on the axial hydroxyl groups were detected, nevertheless, exposure of the resultant mixture to LiOH afforded 18 in excellent yield (87%, three steps). The three axial hydroxyl groups in 18 were then methylated (99%). Unexpectedly, hydrogenolysis of the 400-O-benzyl group in trisaccharide 19 under conventional conditions

O

MPOH

a b & c a

+ 8

b & c a

+ 8

OMP O

HOOAc

OMP

TBDPSO

TBDPSO

+ 8

12 13

14 15

16 R = TBDPS

17 R = H

O

O

O

O

O

TBDPSO

TBDPSO

OMP

HO

O

OMP

OAc

OAc

OAc

O

O

O

O

O

O

RO

O

O

OMP

d, e & f

BnO

RO

O

O

OMP

RO

OAc

OAc

OR

OR

b

g

18 R = H

19 R = Me

h i

+ 4

CAO MeO

OAc

O

O

OCH3

O

OCH3

O

OCH3

5

O

O

O

OR

j & k

20 R = MP

2

Figure 2 | Synthesis of tetrasaccharide donor 2. Highlighted in red are the nascent glycosidic bonds. (a) Ph3PAuNTf2 (0.1 equiv), toluene, 4 MS,

40 C; 95% and b only (for 12); 99% and b only (for 14 and 16); (b) TBAF, THF, 0 C to RT; 99% (from 12); 94% (from 14); 96% (from 16); (c) CH3(OMe)3, p-TsOH, RT, 93% for (13); 91% (for 15); (d) nBu2SnO, MeOH, reux; (e) BnBr, DMF, CsF, RT; (f) LiOH, THF, H2O, RT; 87% (for three steps); (g) MeI, NaH, DMF, 0 C to RT, 99%; (h) Pd(OH)2/C, H2 (1 atm), Et3N, EtOAc, MeOH, 50 C, 93%; (i) Ph3PAuNTf2 (0.2 equiv), toluene, 5 MS,

50 C to RT, 93%, b/a 4/1; (j) Ag(DPAH)2, CH3CN, H2O, 0 C to RT, 95%; (k) o-cyclopropylethynylbenzoic acid, EDCI, DMAP, 4 MS, CH2Cl2,

RT, 99%. DMAP, 4,4-dimethylaminopyridine; DPAH, bis(hydrogen dipicolinate); EDCI, N-ethyl-N0-(3-dimethylaminopropyl)carbodiimide hydrochloride; MS, molecular sieves; TBAF, tetrabutylammonium uoride.

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(Pd(OH)2/C, H2, room temperature (RT)) led to cleavage of the glycosidic linkages, testifying the vulnerability of the cymarosyl-b-(1-4)-linkage. Thus, Et3N was added to sequester any nascent proton; the hydrogenolysis proceeded sluggishly, nevertheless, leading to the desired trisaccharide 5 in a satisfactory 93% yield at 50 C for 2 days.

Given the acid lability of the cymarosyl-b-(1-4)-linkage, it was not fully surprising to nd that glycosylation of trisaccharide acceptor 5 with digitalosyl donor 4 in the presence of Ph3PAuOTf led to considerable cleavage of the trisaccharide. Ph3PAuNTf2 was found to be more stable towards moisture (thus less acidic)27, therefore, it catalysed the condensation of 5 and 4 smoothly. However, in spite of the presence of 2-O-acetyl group in donor 4, the glycosylation led to anomeric mixtures of the coupled tetrasaccharide. Under optimized conditions (0.2 equiv Ph3PAuNTf2, toluene, 5 MS, 50 C to RT), tetrasaccharide

20 was obtained in 93% yield with b/a ratio of 4:1, which was separable on silica gel column chromatography. Removal of the anomeric MP group in tetrasaccharide 20 with CAN was not successful under a variety of conditions, resulting unavoidably degradation of the cymarosyl-b-(1-4)-linkages. Fortunately, a mild oxidizing agent, Ag(DPAH)2, could achieve this task (CH3CN/H2O, 0 C to RT) to afford smoothly the corresponding hemiacetal (95%) (ref. 28), which was then subjected to the formation of ortho-cyclopropylethynylbenzoate 2 (99%) (see Supplementary Methods).

Attempts at construction of the FABO motif. We have tried a number of approaches to the construction of the FABO disaccharide motif, those include condensation of sugar lactones with vicinal diols in the presence of formaldehyde or its surrogates29,30, transacetalation of sugar lactones with sugar 4-hydroxyl-3-methyoxymethyl ether derivatives31, and intra-molecular hydrogen atom transfer reactions of formyl acetal linked disaccharides21,32,33. However, no coupled FABO products have ever been detected, that prompted us to focus our attention on the planned CrichSina approach (Fig. 3). Thus, starting from D-glucal triacetate, 3-O-methyl-6-bromo-glucal 21 and p-methoxyphenyl 2,6-dideoxy-2-iodo-glucoside 11 were prepared in seven steps (66% overall yield) and 13 steps (18% overall yield), respectively (see Supplementary Methods). Glucal 21 was converted into the desired phenylthiomethyl 2-phenylseleno-a-D-mannopyranoside 10 in three steps (45%), that is, addition with PhSeCl to provide 2-phenylseleno-D-

mannopyranose 22, conversion of the lactol into uoride with DAST, and subsequent glycosidation with PhSCH2OH in the presence of SnCl2 (refs 23,34). Condensation of 10 with sugar acceptor 11 under Crichs conditions (NIS, TfOH, CH2Cl2,

30 C) did lead to the desired acetal glycoside 24, albeit in only a moderate yield of B30%; the major product turned out to be the a-glycoside 23 (B65%). A wide variety of the promoters for glycosidation of thioglycosides35 were screened in the present coupling (see Supplementary Table 1), including NBS/TfOH36, Tf2O/BSP/TTBP37, DMTST/TTBP38, MeOTf39 and NIS/

AgOTf40. However, the yield of acetal glycoside 24 was not improved. These results indicate that the transient glycosyloxymethyl cation (generated from 10) decomposes favourably to the glycosyl oxocarbenium species (and a molecule of formaldehyde); capture of the oxocarbenium intermediate by the incoming hydroxyl group (in 11) leads to disaccharide 23. Adjustment of the substituting groups in donor 10, that is, removal of the 6-bromide and/or replacement of the 4-O-benzoyl group with benzyl group also failed to improve the yields of the corresponding acetal glycosides in condensation with 11. Gratifyingly, when we applied the inverse procedure41 (addition

of donor 10 to a mixture of the acceptor 11 and promoter NIS/ TfOH at 30 C) and increased the equivalent of acceptor 11 (to

5.0 equiv), acetal glycoside 24 was obtained in a satisfactory 75% yield. The 4-O-acetyl and 40-O-benzoyl group in 24 were removed simultaneously in the presence of MeONa in MeOH, providing diol 9 (93%), which was ready for Sinas orthoester formation.

Thus, 20-seleno-disaccharide 9 was subjected to oxidation (NaIO4, NaHCO3, MeOH/CH2Cl2/H2O, RT) to provide the selenoxide cleanly, subsequent syn-elimination and intramolecular cyclization of the resultant ketene acetal (A) took place sluggishly under forced conditions (vinyl acetate/toluene/DIPA, 140 C), leading to an orthoester product (25) in a moderate 20% yield for 12 h. By carefully screening the reaction conditions, we nally managed to obtain 25 in an excellent 85% yield under microwave irradiation (145 C, 20 min). The addition of the 4-hydroxyl group onto C10 of the ketene acetal in A could proceed from both the top and the bottom faces, thus two diastereoisomers should be provided. Surprisingly, only one isomer (25) was isolated under various conditions. We had expected that the diastereoselectivity bestowed by the two sugar units could lead to formation of the native conguration in the natural product (opposite to that drawn in 25). However, in the previous synthesis of the Sina-type ve- and six-membered orthoesters, cyclization of the incipient ketene acetals was found to favour formation of the axial a-linkage, so as to maximize the anomeric effect2224 or to follow the trajectory of addition onto Woerpels low-energy conformer of the dioxocarbenium intermediate42,43. Determination of the conguration of the quaternary C10 in 25 was not possible by spectroscopic methods, especially without comparison to its epimer, and attempts at acquisition of a single crystal of 25 or its derivatives for X-ray diffraction analysis were unsuccessful. Therefore, this problem was not solved until completion of the total synthesis.

Synthesis of C100-epi-periploside A (31). Temporary protection of the 40-OH in 25 with benzoyl group led to 26 (99%), which was subjected to selective cleavage of the anomeric MP group (Ag(DPAH)2, CH3CN, H2O, 90%) and subsequent formation of triuoroacetimidate (95%) to afford the desired donor 27 (Fig. 3). Glycosylation of pregnane diol 7, which was prepared from hydroxyandrost-5-en-17-one in three steps (see Supplementary Methods and Supplementary Fig. 59), with disaccharide imidate 27 proceeded smoothly under the catalysis of TBSOTf (0.1 equiv) in the presence of 5 MS at 78 C in CH2Cl2, affording pregnane

20-O-disaccharide 28 in 85% (96%, b.r.s.m.) yield and b/a ratio of 3:1. The erosion of 1,2-trans-selectivity in the glycosylation with a donor (that is, 27) equipped with an iodide at C2 could be contributed to the presence of the FABO motif, which might cause conformational restraint for the neighbouring participation. Notably, the present reaction must be quenched at 78 C

(with Et3N), so as to avoid the decomposition of the acid-labile FABO motif. Reductive removal of the bromide and iodide in 28 under the conventional radical conditions (AIBN/Bu3SnH, toluene, 80 C) led to decomposition of the substrate. Et3B could initiate the radical reaction at RT44, which thus enabled the reduction of 28 with Bu3SnH to proceed smoothly to afford the corresponding deoxydisaccharide (99%). Subsequent removal of the 40-O-benzoyl group provided the desired pregnane 20-O-disaccharide 29 (99%).

The expected challenge in stereoselective construction of the 2-deoxy-b-cymarosyl-(1-4)-linkage in the union of tetrasaccharide 2 and pregnane disaccharide 29 was further manifested by the fact that both the 2,6-dideoxyglycosidic linkages and the FABO motif were shown to be extremely labile toward acid. Thus, we screened carefully the coupling conditions, including the gold(I)

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Br

SePh

Br

SePh

a b & c

O

O

d

BzO

MeO

Br

O

BzO

MeO

BzO

MeO

OH

+ 11

21 22 10

24 R1 = Ac, R2 = Bz

9 R1 = R2 = H

28 29

OCH2SPh

a

Br

Br

O

O

O

BzO

MeO

SePh

O

R2O

MeO

SePh

O

O

R1O

O

I

f & g

AcO

O

OMP

OMP

+

O

HOO

I

H+

b

23

e

A

Br

Br

O

O

BzO

MeO

RO

MeO

O

i & j

O

O

O

O

I

O

O

I

OMP

O NPh CF3

O

27

h 25 R = H

26 R = Bz

Br

O

O

BzO

MeO

HO

MeO

O

I

O

O

O

k

O

O

O

OH l & m

O

O

O

OH

+ 7

TBSO

TBSO

O

n

+ 2

o & p

CAO MeO

OAc

O

OMe

O

OMe

O

OMe

O

O

OO

O

O

O

O

O

Me

O

O

OH

30

TBSO

HO MeO

OAc

O

OMe

O

O

O

O

O

O

OMe

O

OMe

O

O

OO

O

Me

1

O

O

1

OH

C1-epi-periploside A (31)

HO

Figure 3 | Construction of the FABO motif and synthesis of C100-epi-periploside A (31). Highlighted in red are the nascent glycosidic bonds. (a) PhSeCl, CH3CN, 40 C, 78%; (b) DAST, THF, 30 C to RT; (c) PhSCH2OH, SnCl2, CH2Cl2, 4 MS, 40 C to RT; 58% (for two steps); (d) NIS, TfOH,

CH2Cl2, 30 C, 75% (for 24), 20% (for 23); (e) MeONa, MeOH, CH2Cl2, RT, 93%; (f) NaIO4, NaHCO3, MeOH, CH2Cl2, H2O, RT, 99%; (g) vinyl

acetate, toluene, DIPA, Mw, 145 C, 20 min, 85%; (h) BzCl, Et3N, DMAP, CH2Cl2, 0 C to RT, 99%; (i) Ag(DPAH)2, CH3CN, H2O, 0 C to RT, 90%; (j) N-phenyl-2,2,2-triuoroacetimidoyl chloride, Cs2CO3, CH2Cl2, RT, 95%; (k) TBSOTf, CH2Cl2, 5 MS, 78 C, 85%, b/a 3/1; (l) Et3B, Bu3SnH,

toluene, RT, 97%; (m) MeONa, MeOH, CH2Cl2, RT, 99%; (n) Ph3PAuOTf (0.8 equiv), TTBP, CH2Cl2, 4 MS, 20 C to 10 C, 64% (87% b.r.s.m.),

b/a 2.1/1; (o) thiourea, pyridine, EtOH, 80 C; (p) HF py, pyridine; THF, 0 C to RT; 91% (for two steps). DAST, (diethylamino)sulfur triuoride;

DIPA, diisopropylamine; TBSOTf, tert-butyldimethylsilyl triuoromethane sulfonate; Mw, microwave; TTBP, 2,4,6-tri-tert-butylpyrimidine.

catalyst, solvent and temperature. When the coupling of 2 and 29 was conducted in the presence of Ph3PAuNTf2 (0.2 equiv), the coupled hexasaccharide was obtained in good yield (50%) but in favour of the thermodynamically more stable a-anomer (b/aB1:3). With Ph3PAuOTf as the catalyst, however, the reaction of 2 and 29 provided a messy mixture. Careful isolation led to identication of a pentasaccharide lactone, which was derived from cleavage of the FABO linkage in the coupled hexasaccharide (30). Encouragingly, the originally formed cymarosyl-(1-4)-linkage in the resultant pentasaccharide lac-tone was found in the required b conguration, implying that the

glycosylation reaction took place via a glycosyl a-triate intermediate18. Nevertheless, the HOTf generated after glycosylation, before being quenched by the isochromen-4-yl gold(I) complex45, degraded the FABO linkage. On the basis of this rational, we introduced a hindered base, that is, 2,4,6-tri-tertbutylpyrimidine (TTBP), into the present Ph3PAuOTf-catalysed glycosylation to rest the incipient HOTf, so as to avoid the cleavage of the FABO linkage. The sequester of the HOTf also retarded the gold(I) catalytic cycle, therefore, requiring almost equivalent of the gold complex to drive the reaction to completion45,46. In fact, the condensation of 2 and 29 proceeded

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smoothly in the presence of Ph3PAuOTf (0.8 equiv) and TTBP(1.5 equiv) in CH2Cl2 at 10 C, leading to the coupled

hexasaccharide 30 in a satisfactory yield of 64% (87%, b.r.s.m.) and b/a ratio of 2.1:1. Finally, removal of the terminal CA group and TBS group was achieved with thiourea47 and pyridine-buffered HF pyridine, respectively, furnishing the target

pregnane hexasaccharide 31 cleanly (91%, two steps).

The 1H and 13C NMR spectra of 31 are similar to those of the authentic periploside A (1) (see Supplementary Figs 60 and 61). However, discrepancies occur for the signals from the formyl acetyl CH2 residue (88.4 p.p.m. for the 13C signal in 31 versus86.4 p.p.m. in 1; 4.93 and 4.82 p.p.m. for the 1H signals in 31 versus 5.13 and 4.74 p.p.m. in 1) (see Supplementary Table 3). In addition, the adjacent C40, C200 and C300 are also in disparate chemical shifts (C40: 81.5 versus 79.2 p.p.m.; C200: 37.9 versus36.7 p.p.m.; C300: 77.4 versus 78.3 p.p.m., in 31 and 1, respectively). These discrepancies indicate that the synthetic 31 is indeed the epimer of periploside A (1) with the opposite conguration at the quaternary C100. The problem of diastereoselectivity in the previous formation of the FABO motif is thus addressed.

Construction of the FABO motif of the natural conguration. The addition of the hydroxyl group onto the ketene acetal in A proceeded exclusively from the a face, leading to the FABO disaccharide with the unnatural conguration (9-25). The presence of a nucleophile capable of interception of the oxocarbenium species developed from the ketene acetal might lead to a thermodynamically favored a-intermediate; substitution of the intermediate in situ by the 4-hydroxyl group would then proceed from the b face to provide the FABO disaccharide with the natural conguration. Therefore, we tried the elimination/cyclization (from 9) in various nucleophilic solvents, including CH3CN, 1,4-dioxane, THF, DME, DMF and MeOH, under varied

temperatures; however, the only FABO disaccharide identied was 25. Addition of nucleophilic additives, such as 4-dimethylaminopyridine (DMAP), LiBr, NaBr and NaI, was also found futile. The presence of an electrophilic reagent, such as NIS, NBS and I2, might convert the ketene acetal into a 1,2-halonium intermediate, which could then be attacked by the 4-hydroxyl group to give the FABO disaccharide. These attempts were again unsuccessful.

The failure in formation of the seven-membered orthoester in the desired stereochemistry forced us to construct the orthoester before cyclization of the formyl acetal (Fig. 4). Thus, 2-phenylseleno-D-mannopyranoside 22 was converted into the uoride (with DAST), which was then coupled with sugar acceptor 32 (see Supplementary Methods) under the action of SnCl2 to give a-disaccharide 33 (85%). Gratifyingly, after intensive attempts, we managed to obtain the ketene acetal 34 in excellent yield (91%) from disaccharide 33 via selenoxide formation and syn-elimination under the modied Sina conditions (NaIO4, NaHCO3, MeOH/CH2Cl2/H2O, RT; then vinyl acetate/toluene/DIPA, microwave 140 C, 40 min). Although purication of 34 on silica gel required the addition of 1% Et3N in the eluent to prevent hydrolysis, the puried ketene acetal 34 remained stable at 20 C for several days. To the best

of our knowledge, this is the rst time a ketene acetal linked disaccharide (that is, 34) being isolated. Noteworthy is the decisive role played by the 3-O-Lev group (in 3335), which facilitated the procurement of the ketene acetal disaccharide as well as the selective removal afterwards; in contrast, analogues of 33 bearing an electron-donating group (for example, TBS) at the 3-OH led to decomposed monosaccharide derivatives under identical conditions.

Addition of PhSCH2OH onto ketene acetal 34 was rst attempted in CDCl3 at 50 C (ref. 48), the starting ketene acetal decomposed largely in 12 h, with the desired orthoester being isolated in low yield (20%) as a single a-isomer. By raising the

Br

Br

O

O

a b

BzO

MeO

SePh

BzO

MeO O

O

LevO OMP

c & d

22

O

LevO OMP

O

I

HO

LevO

32

O

I

OMP

33

I

34

Br

Br

e

BzO

MeO

O

O OMP

O

LevO

O

BzO

MeO

f

O OMP

O

HO

I

I

O

O

35 36

SEt

SEt

CH2O

+

O

O

g

O HO

O HO

+

O

B

C

Br

BzO

MeO

O

O OMP

I

O

Br

O

O

O

O

O

BzO

MeO

OMP

O

I

37

38

Figure 4 | Construction of the FABO motif with the natural conguration. Highlighted in red are the nascent glycosidic bonds. (a) DAST, THF, 30 C to

RT; (b) SnCl2, Et2O, 4 MS, 0 C to RT; 85% (for two steps); (c) NaIO4, NaHCO3, MeOH, CH2Cl2, H2O, RT, 99%; (d) vinyl acetate, toluene, DIPA, Mw, 140 C, 40 min, 92%; (e) EtSCH2OH, DCCl3, Mw, 10 min, 110 C, 81%; (f) H2NNH2 H2O, pyridine, HOAc, 0 C to RT, 92%; (g) BSP, Tf2O, DTBP,

5 MS, Et2O, 114 C, 64% (for 37), 18% (for 38). BSP, 1-benzenesulnyl piperidine; DTBP, 2,6-di-tert-butylpyridine; Lev, levuloyl; Mw, microwave.

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NATURE COMMUNICATIONS | DOI: 10.1038/ncomms6879 ARTICLE

temperature and shortening the reaction duration (CDCl3,

microwave 100 C, 1 h), the addition of 34 and PhSCH2OH led to the desired orthoester in a good 70% yield but in a moderate diastereoselectivity of 1.4/1. Modication of the reaction conditions by the addition of acidic promoters (p-TsOH or PPTS) or variation of solvent (toluene, CH2Cl2 or CHCl3) failed to improve the yield or the diastereoselectivity. Fortunately, replacement of PhSCH2OH with the more nucleophilic

EtSCH2OH, the addition with ketene acetal 34 under the optimal conditions (CDCl3, microwave 110 C, 10 min) furnished the desired orthoester 35 in 81% yield as a single a-isomer. It should be noted that the replacement of CDCl3 with

CHCl3 or toluene led to lower yields of 35 (o65%). Selective removal of the 3-O-Lev group in 35 was achieved with H2NNH2 H2O to provide orthoester 36 (92%).

Treatment of ethylthiomethyl glycoside 36 with the mild promoters for glycosidation of thioglycosides (see Supplementary Table 2), such as MeOTf/TTBP, DMTST/TTBP, and CuBr2/

Bu4NBr49, failed to afford the seven-membered FABO derivative 37; instead, the ve-membered orthoester 38 was isolated in high yield (480%) as a mixture of the two diastereoisomers. These results indicate again (cf., 10-23/24) that the glycosyloxymethyl cation (B) generated via activation of the thioacetal could readily undergo decomposition to the glycosyl oxocarbenium (C) and formaldehyde; intramolecular addition of the proximal hydroxyl group to C led to the ve-membered orthoester. Thus, a strong promoter which can activate the thioacetal under milder conditions might be able to allow the transient glycosyloxymethyl cation B to be captured by the hydroxyl group before decomposition. Using Crichs conditions (Tf2O/BSP/TTBP,

60 C, CH2Cl2)37, however, the ve-membered orthoester 38 was again obtained nearly quantitatively as a mixture of the diastereoisomers. Encouragingly, when lowering the reaction temperature to 78 C, a trace amount of the desired seven-

membered FABO product 37 was detected. Optimizing along this direction, we nally managed to obtain the desired 37 in a

satisfactory 64% yield in the presence of Tf2O/BSP/DTBP in Et2O at 114 C, whereas the ve-membered orthoester 38 was

isolated in 18% yield as a single diastereoisomer. Comparison of the NMR data of the present FABO disaccharide 37 with those of the previous 26 supported that we had xed the desired conguration by the present approach.

Completion of the synthesis of periploside A (1). The transformations previously developed for the synthesis of C100-epiperiploside A (26-31, eight steps, 28% overall yield) were applied to the synthesis of periploside A (Fig. 5). Thus, FABO disaccharide 37 was subjected to selective cleavage of the anomeric MP group (with Ag(DPAH)2, 91%) and conversion into the triuoroacetimidate donor 6 (90%). Coupling of pregnane diol 7 with donor 6 under the similar conditions as that for 7 27-28 (85%, b/a 3:1) led to the corresponding dis

accharide 39 in a similar yield (87%) but much higher b selectivity (b/a 6.1:1). This result supports the previous assumption

that the conformational restraint provided by the FABO motif affects the glycosidation transition state of the disaccharide. The bromide and iodide in 39 were removed cleanly with Et3B/

Bu3SnH (95%); subsequent cleavage of the 40-O-benzoyl group (NaOMe, HOMe, 96%) provided the desired disaccharide acceptor 3. Condensation of 3 with tetrasaccharide donor 2 under the optimized conditions for 29 2-30 (64%, b/a 2.1:1)

afforded hexasaccharide 40 in a higher 80% (92%, b.r.s.m.) yield and similar b/a ratio of 2:1. Finally, the terminal CA and TBS groups were removed successfully with thiourea and pyridine-buffered HF-pyridine, respectively, furnishing the target periploside A (1) (93%, two steps). Gratifyingly, all the analytical data of 1 are in full agreement with those obtained for the natural product1 (see Supplementary Table 3).

The immunosuppressive activities of the synthetic compounds. The synthetic periploside A (1) showed similar toxicity and

Br

O

a & b

NPh

O

c

BzO

MeO

O

O

O

O

O

OMP

O I

I

+ 7

O

OH

I

CF3

37 6

TBSO

39

O

HO

MeO

O

O

O

O

d & e

O

OH

f

+ 2

TBSO

3

1

RO O

O

O

O

O

O

O

O

O

OO

O

O

O

1

O

O

O

O

O

1

O

O

OH

g & h

40 R = CA, R1 = TBS

Periploside A (1) R = R1 = H

R1O

Figure 5 | Completion of the total synthesis of periploside A (1). Highlighted in red are the nascent glycosidic bonds. (a) Ag(DPAH)2, CH3CN, H2O, 0 C, 91%; (b) N-phenyl-triuoroacetimidoyl chloride, Cs2CO3, CH2Cl2, RT, 90%; (c) TBSOTf, CH2Cl2, 5 MS, 78 C, 87%, b/a 6.1/1; (d) Et3B,

Bu3SnH, toluene, RT, 95%; (e) MeONa, MeOH, CH2Cl2, RT, 96%; (f) Ph3PAuOTf (0.8 equiv), TTBP, CH2Cl2, 4 MS, 10 C, 80%, b/a 2/1; (g)

thiourea, pyridine, EtOH, 80 C; (h) HF py, pyridine, THF, 0 C to RT, 93% (for two steps).

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Table 1 | Inhibitory activity of periploside A and analogues against T-lymphocyte proliferation*.

Compound CC50 (lM) IC50 (lM) SI

Periploside A (1) 2.100.32 0.170.04 12 C100-epi-periploside A (31) 1.580.19 0.410.15 3.9

C1000-epi-periploside A (41) 11.403.66 1.960.43 5.8

Disaccharide 42 12.800.52 6.203.20 2.1

Disaccharide 43 27.706.61 3.702.25 7.5

*See Supplementary Methods and Supplementary Figs 62 and 63 for details.

41

HO O

O O

OO

O

O O

O

O

O O

O O

O

O

1'''

O

O

O O

O

OH

HO

O

O

1'

HOO

O

O

O

1'' O

O

O

O

O

HO O O

OH

O

OH

HO

HO

42 43

Figure 6 | Synthetic analogues of periplosides. Shadowed in pale blue are the carbon centres with opposite congurations to those in the nature product.

activity as the natural product against T-lymphocyte and their proliferation induced by ConA5,6. The C100-epimer (31) which has the opposite conguration at the FABO motif as in periploside A was also found active (IC50 0.41 mM), although

being B2.4-fold less potent than the natural product (Table 1). The C1000-epimer of periploside A (41) was also active (IC50 1.96 mM) (Fig. 6). Interestingly, disaccharide 42, with

the tetrasaccharide in 31 being truncated, still had certain activity (IC50 6.20 mM); and its a-anomer 43 even showed a higher

activity (IC50 3.70 mM). Previous assays have demonstrated that

reductive cleavage of the formyl acetal in the FABO motif in periploside A abolished the activity completely6. Taken together, it demonstrates that the chemical connection of the FABO motif, rather than the stereochemistry, has a critical role in the immunosuppressive activities of periplosides. The capability of releasing a formylaldehyde might be taken into account in the future researches into the mechanism of action of this unique type of compounds.

Methods

General methods. All the reactions were carried out under nitrogen or argon with anhydrous solvents in ame-dried glassware, unless otherwise noted. All the glycosylation reactions were performed in the presence of 4 or 5 MS, which were ame-dried immediately before use in the reaction under high vacuum. Glycosylation solvents were dried using a solvent purication system and used directly without further drying. The chemicals used were reagent grade as supplied, except where noted. For details of the synthetic procedures and the characterization data of compounds, see Supplementary Methods. For 1H and 13C NMR spectra of the compounds prepared in this study, see Supplementary Figs 158.

Synthesis of acetal glycoside 24. To a solution of sugar alcohol 11 (620 mg,1.47 mmol) in CH2Cl2 (5 ml) was added acid-washed 3 MS at RT. After stirring

for 30 min at RT, NIS (142 mg, 0.63 mmol) and TfOH (2.6 ml, 0.029 mmol) were added to the mixture at 30 C, followed by the addition of a solution of phe

nylthiomethyl glycoside 10 (183 mg, 0.29 mmol) in CH2Cl2 (3 ml) via a syringe pump. The reaction mixture was stirred at 30 C for 1 h. When TLC showed the

donor 10 had been consumed, saturated aqueous NaHCO3 was added at 0 C. The mixture was ltered. The ltrate was washed with a solution of NaS2O3 and brine, respectively, and was then dried over Na2SO4 and concentrated. The residue was puried by ash chromatography (petroleum ether/CH2Cl2/EtOAc 8:1:1) to

afford 24 (206 mg, 75%) and glycoside 23 (53 mg, 20%) as syrups.

Synthesis of FABO disaccharide 25. To a solution of acetal glycoside 9 (187 mg,0.24 mmol) in MeOH/CH2Cl2/H2O (3 ml/2 ml/1 ml) were added NaIO4 (507 mg,2.37 mmol) and NaHCO3 (159 mg, 1.90 mmol) at RT. After stirring for 3 h, the mixture was diluted with CH2Cl2, washed with saturated NH4Cl solution and brine, respectively, and was then dried over Na2SO4 and concentrated. The resultant selenoxide was azeotroped with toluene (3 5 ml) and dried under high

vacuum for 2 h to afford a white solid (190 mg, 99%). The above selenoxide(125 mg, 0.155 mmol) was dissolved in toluene (6 ml). Diisopropylamine (3 ml) and vinyl acetate (6 ml) were added, and the reaction was conducted under microwave at 145 C for 20 min. The mixture was cooled to RT and concentrated. The residue was puried by ash chromatography on silica gel (petroleum ether/EtOAc 1.5:1)

to afford 25 (83 mg, 85%) as a colourless syrup.

Synthesis of a-disaccharide 33. To a solution of lactol 22 (603 mg, 1.21 mmol) in

THF (10 ml) was added DAST (0.44 ml, 3.63 mmol) at 30 C. After stirring for

1.5 h while warming to RT, a saturated NaHCO3 solution was added slowly to the mixture. The resulting mixture was extracted with CH2Cl2. The combined organic layer was washed with brine, dried over Na2SO4 and concentrated. The crude glycosyl uoride was azeotroped with toluene (3 5 ml). After drying under high

vacuum for 2 h, the above product was dissolved in Et2O (10 ml), 4 MS (1.2 g) and sugar alcohol 32 (330 mg, 0.69 mmol) were added and the reaction mixture was stirred at 0 C for 30 min. SnCl2 (235 mg, 1.24 mmol) was added in one portion and the reaction mixture was allowed to warm to RT and stirred for 4 h. The mixture was quenched with Et3N (1 ml) and ltered. The solution was diluted with

EtOAc and washed with water. The water layer was extracted with EtOAc twice. The combined organic layer was washed with saturated NaHCO3 solution and brine, respectively, and was then dried over Na2SO4 and concentrated. The residue was puried by ash chromatography (petroleum ether/EtOAc 4:1) to afford 33

(560 mg, 85%) as a colourless syrup.

Synthesis of ketene acetal 34. To a solution of 33 (248 mg, 0.26 mmol) in MeOH/CH2Cl2/H2O (3 ml/2 ml/1 ml) were added NaIO4 (552 mg, 2.58 mmol) and NaHCO3 (173 mg, 2.06 mmol) at RT. After stirring for 12 h at RT, the mixture was diluted with CH2Cl2, and washed with saturated NH4Cl solution and brine, respectively. The organic layer was dried over Na2SO4 and concentrated. The crude selenoxide was azeotroped with toluene (3 5 ml) and dried under high vacuum

for 2 h to afford a colourless syrup (251 mg, 99%). The above selenoxide (104 mg,0.11 mmol) was dissolved in toluene (2 ml). Diisopropylamine (1 ml) and vinyl acetate (2 ml) were added. The reaction was conducted under microwave at 140 C for 40 min. The mixture was cooled to RT and concentrated. The residue was puried by ash chromatography (petroleum ether/EtOAc 5:1, containing 1%

Et3N) to afford 34 (85 mg, 92%) as a colourless syrup.

Synthesis of orthoester 35. To a solution of 34 (75 mg, 0.093 mmol) in CDCl3 (3 ml) was added EtSCH2OH (0.05 ml) at RT. The reaction was conducted under microwave at 110 C for 10 min. The mixture was cooled to RT and concentrated. The residue was puried by ash chromatography (petroleum ether/EtOAc 5:1, containing 1% Et3N) to afford 35 (67 mg, 81%) as a colourless

syrup.

Synthesis of orthoester 36. To a solution of 35 (110 mg, 0.120 mmol) in pyridine/HOAc (3 ml/2 ml) was added H2NNH2 H2O (0.10 ml, 1.60 mmol) at 0 C. After stirring at RT for 5 h, the mixture was diluted with CH2Cl2, and washed with ice water and then with a saturated NaHCO3 solution and brine, respectively. The organic layer was dried over Na2SO4 and concentrated. The residue was puried by ash chromatography (petroleum ether/EtOAc 5:1, containing 1% Et3N) to

afford 36 (90 mg, 92%) as a colourless syrup.

Synthesis of FABO disaccharide 37. To a solution of 36 (19.1 mg, 0.024 mmol) in Et2O (3 ml) were added BSP (8.2 mg, 0.036 mmol), 2,6-di-tert-butylpyridine (16.0 ml,0.072 mmol) and 5 MS at RT. After stirring at 114 C (liq. N2-EtOH) for

20 min, Tf2O (6.0 ml, 0.036 mmol) was added to the mixture. The mixture was stirred at 114 C for 1 h, and was then warmed to RT and ltered. The ltrate was

washed with a saturated aqueous NaHCO3 solution and brine, respectively, and was then dried over Na2SO4 and concentrated. The residue was puried by ash chromatography on silica gel (petroleum ether/EtOAc 5:1) to afford 37 (11.3 mg,

64%) and the ve-membered orthoester 38 (3.0 mg, 18%) as colourless syrups.

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Synthesis of FABO disaccharide triuoroacetimidate 6. To a solution of p-methoxyphenyl glycoside 37 (36 mg, 0.049 mmol) in CH3CN/H2O (3 ml/3 ml)

was added Ag(DPAH)2 (79 mg, 0.17 mmol) at 0 C. After stirring for 30 min at this temperature, the mixture was ltered. The ltrate was diluted with CH2Cl2, washed with saturated NaHCO3 solution and brine, respectively, and was then dried over Na2SO4 and concentrated. The residue was puried by ash chromatography (petroleum ether/EtOAc 3:1) to yield the corresponding hemiacetal

(28 mg, 91%) as a colourless syrup. To a solution of the hemiacetal (29 mg,0.046 mmol) in CH2Cl2 (3 ml) were added Cs2CO3 (75 mg, 0.23 mmol) and N-phenyl-2,2,2-triuoroacetimidoyl chloride (14 ml, 0.14 mmol) at RT. After stirring for 3 h, the mixture was ltered. The ltrate was evaporated in vacuo to give a residue, which was subjected to chromatography on Davisil silica (pH 7.0, pet

roleum ether/EtOAc, 5:1) to give 6 (33 mg, 90%) as a colourless syrup. This compound was used directly without further characterization.

Synthesis of pregnane b-disaccharide 39. To a solution of imidate 6 (33.0 mg,0.041 mmol) and pregnane diol 7 (15.6 mg, 0.035 mmol) in CH2Cl2 (3 ml) was added 5 MS at RT. After stirring at 78 C for 30 min, TBSOTf (1.2 ml,

0.0052 mmol) was added to the mixture. After stirring for 6 h at this temperature, Et3N was added to quench the reaction. The resulting mixture was ltered. The ltrate was evaporated in vacuo to give a residue, which was puried by ash chromatography (petroleum ether/CH2Cl2/EtOAc 10:5:1) to afford 39 (27.6 mg,

75%) and its a-anomer (4.5 mg, 12%) as white solids.

Synthesis of pregnane disaccharide 3. To a solution of 39 (21.0 mg, 0.020 mmol) in toluene (2 ml) were added Bu3SnH (32 ml, 0.12 mmol) and Et3B (12 ml,0.012 mmol) at 0 C. After stirring for 1 h at RT, the mixture was concentrated in vacuo. The residue was puried by ash chromatography (petroleum ether/ EtOAc 5:1) to afford the corresponding 20,600-deoxy derivative (16.5 mg, 97%) as

a white solid (see Supplementary Methods). To a solution of this compound(16.5 mg, 0.019 mmol) in CH2Cl2/MeOH (1.5 ml/1.5 ml) was added NaOMe(20 mg, 0.37 mmol) at RT. After stirring for 40 h, the mixture was ltered through silica gel. The ltrate was evaporated in vacuo to give a residue, which was puried by ash chromatography (petroleum ether/EtOAc 2:1) to afford 3 (14.0 mg, 97%)

as a white solid.

Synthesis of pregnane hexasaccharide 40. To a solution of tetrasaccharide ortho-cyclopropylethynylbenzoate 2 (22.3 mg, 0.025 mmol), pregnane disaccharide 3 (8.0 mg, 0.011 mmol) and 2,4,6-tri-tert-butylpyrimidine (TTBP) (4.0 mg,0.016 mmol) in CH2Cl2 (2 ml) was added 4 MS at RT. After stirring for 30 min at

20 C, a solution of PPh3AuOTf in CH2Cl2 (0.05 ml, 0.1 M) was added to the mixture. The mixture was stirred for 2 h while warming to 10 C, then another

portion of PPh3AuOTf in CH2Cl2 (0.05 ml, 0.1 M) was added to the mixture. After stirring for 4 h at 10 C, Et3N was added to quench the reaction. The resulting

mixture was ltered and concentrated. The residue was puried by ash chromatography (petroleum ether/CH2Cl2/EtOAc 1:1:1) to afford 40 (8.3 mg, 53%),

its a-anomer (4.2 mg, 27%) as white foams, and recovered 3 (1.0 mg, 13%).

Synthesis of Periploside A 1. To a solution of 40 (4.7 mg, 3.2 mmol) in pyridine/ EtOH (1.0 ml/1.0 ml) was added thiourea (10 mg, 0.13 mmol) at RT. After stirring for 2 h at 80 C, the mixture was concentrated in vacuo to give a residue, which was puried by ash chromatography (CHCl3/MeOH 30:1) to afford a colourless

syrup. The syrup was dissolved in THF/pyridine (1.5 ml/0.75 ml). HF-py (70% HF in pyridine, 0.10 ml) was added dropwise at 0 C. After stirring for 40 h at RT, a saturated NaHCO3 solution was added slowly to the mixture at RT. The resulting mixture was diluted with CH2Cl2, washed with saturated NaHCO3 solution and was then extracted with CH2Cl2 twice. The combined organic layer was washed with brine, dried over Na2SO4 and concentrated. The residue was puried by ash chromatography (CHCl3/MeOH 30:1) to afford periploside A (1) (3.8 mg, 93%)

as a white foam.

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Acknowledgements

This work is nancially supported by the National Natural Science Foundation of China

(21432012 and 91213301), the Ministry of Sciences and Technology of China

(2012ZX09502-002) and the E-Institute of Shanghai Municipal Education Commission

(E09013). We are grateful to Professor Wei-Min Zhao for providing an authentic sample

of the natural product periploside A and to Professor Tian-Xiang Li for providing a

photo of the plant.

Author contributions

X.Z. and B.Y. conceived the synthetic route. X.Z. conducted the synthetic work. Y.Z. and

J.Z. conducted bioassay. B.Y. and X.Z. wrote the manuscript.

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How to cite this article: Zhang, X. et al. Total synthesis of periploside A, a unique

pregnane hexasaccharide with potent immunosuppressive effects. Nat. Commun. 6:5879

doi: 10.1038/ncomms6879 (2015).

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