Suppl Figures + Tables-compressed.pptx - Nature

1.5

0.25 ng

165 ng

2  

3  

Tet2/3 DKO

Tet3 KO

Spleen (4 wk after injection)

N.D.

5 μg

Standard

Tet2/3 DKO

Tet3KO

Tet2KO

WT

Tet2/3 DKO

Tet3KO

0.5 ng

e

5 μg

0.5 ng

4  

Two-fold serial dilutions

LSK CMP GMP MEP 2 1.5 anti-5hmC Anti-5hm

anti-5hmC Anti-5h

anti-5hmC

1  

2  

3  

N.D.

0

N.D.

0.5

N.D.

1 N.D.

Tet3 mRNA levels (relative to Gapdh)

Tet2 KO

anti-CMS

Two-fold serial dilutions

1  

N.D.

N.D.

N.D.

0

Tet2KO

d

0.8

WT

1.2

Standard

1.6

0.4

WT

anti-CMS

Tet2/3 DKO

anti-CMS

Bone marrow Spleen (2 wk after injection)

Tet3KO

LSK CMP GMP MEP

Two-fold serial dilutions

4  

Tet2KO

3  

165 ng

WT

2  

0.25 ng

Two-fold serial dilutions

0.5 1  

Standard

Tet2/3 DKO

Tet3 KO

Tet2 KO

WT

c

1

0

Tet2 mRNA levels (relative to Gapdh)

Tet2/3 DKO

DKO

Tet3 KO

WT

2

Tet2 KO

b

WT

Tet1 mRNA levels (relative to Gapdh)

a

Standard

Supplementary Fig. 1

4  

LSK CMP GMP MEP

Spleen Spleen (4 wk after injection) (2 wk after injection)

Bone marrow (4 wk after injection)

Supplementary Figure 1. Loss of genomic 5hmC in hematopoietic cells of Tet2/3 DKO mice. (a) Expression of Tet1, Tet2 and Tet3 in sorted LSK and myeloid progenitor cells. Cells were isolated from bone marrow of WT (Tet3fl/fl) or DKO (Tet2-/- Tet3fl/fl Mx1-Cre+) mice at 2 weeks after pIpC administration by flow cytometry, and quantitative RT-PCR was performed. The relative levels of mRNAs after normalization to the level of Gapdh mRNA in the same cell population are shown, with the amount in the WT LSK cells arbitrarily set to 1. N.D., not detected. (b-e) Quantification of 5hmC levels in cells from Tet2/3 DKO mice. (b, c) At two (b) or four (c) weeks following pIpC administration, 5hmC levels in the bone marrow or spleen were quantified by dot blot assay with anti-CMS antibody after treatment of genomic DNA with bisulfite. A synthetic oligonucleotide with a known amount of CMS was used as standard. (d, e) Top panels, At two or four weeks following pIpC administration, 5hmC levels in the spleen (d) or bone marrow (e) were quantified by dot blot assay with anti-5hmC antibody (top panels). Bottom panels, Methylene blue staining was used to monitor equivalent DNA loading. A synthetic oligonucleotide with a known amount of 5hmC was used as standard.

Supplementary Fig. 2

Hematocrit (%)

***

*

*

**

*

**

40 20

7

14 28

Days post-injection

nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l O

0

Pre 0/2

7

Pre 0/2

7

14 28

Days post-injection

Platelets/μl (X 106)

0 nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l O

Pre 0/2

14 28

Pre 0/2

7

14 28

Days post-injection

Days post-injection

g 60

*** ***

0.5 500

Co

14 28

f *

0

Days post-injection

Co

Hemoglobin (g/dL)

e

*

*

h

15

**

**

**

*

**

10 5 0

Pre 0/2

7

14 28

Days post-injection

50 40 30 20

**

10

** *

** *

0 nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l O

Days post-injection

7

1

Lymphocytes/μl (X103)

Pre 0/2

**

2

***

10001

Co

14 28

3

nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l O

nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l O

7

0 Co

Co

Pre 0/2

10

1500 1.5

*

nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l O

0

*

4

Basophils/μl (X103)

5

20

d

Co

10

*

30

Red blood cells/μl (X106)

15

c

Co

**

20

Eosinophils/μl (X103)

b

WT DKO

nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l Co O nt ro DK l O

Monocytes/μl (X103)

a

Pre 0/2

7

14 28

Days post-injection

Supplementary Figure 2. Hematopoietic cell numbers in peripheral blood of WT and Tet2/3 DKO mice. (a-g) Time-course analysis of peripheral blood cell counts. Tet2/3 DKO mice developed progressive monocytosis (a), eosinophilia (b), basophilia (c), thrombocytopenia (d) and anemia (e-g). (h) There was a slight decrease in lymphocyte numbers in the peripheral blood of DKO mice after pIpC injection although the difference at day 28 was not statistically significant (n = 7~10 per each genotype at each time point examined). Means ± SEM are shown. *P < 0.05, **P < 0.005, ***P < 0.0005 (Student's t test).

Supplementary Fig. 3

b

c ** **

50

0/2

DK O

rl ct 4w

k

rl ct 1w

on m 02

k

ct

rl

0 PI

28

DK O

25 o

DK O

rl ct

75

4w

7

Days post-injection

d

100

Percentage

Days post-injection

k

rl 1w

an gr

0/2

2

28

0/

7

DK O

ct

ct

rl

DK O

0

4w

k

DK O

rl ct k

25

PI

0/2

C

0/2

D

50

D

D

11

1w

b+

ctr

l

0

DK O

25

***

75

ct

50

Mac-1+Gr-1-

***

k

Percentage

75

***

100

DK O

***

l

***

ro

***

100

Percentage

Mac-1+Gr-1+

D

Mac-1+

DK O

a

7

28

Days post-injection

e B220+CD19+

DK O

rl ct k 4w

DK O

rl 1w

ce T

4w

ct

0

k

DK O

rl ct k

rl ct k

Days post-injection

02

28

PI

7

WT DKO

10

D

02 PI D

0/2

***

20

B

1w

ce

ll

ct

rl

0

DK O

20

***

DK O

40

30

rl

Percentage

60

***

40

***

ct

***

ll

***

DK O

Percentage

80

CD4+/CD8+

0/2

7

28

Days post-injection

Supplementary Figure 3. Expansion of myeloid lineage cells with decrease in lymphoid lineage cells in Tet2/3 DKO mice. (a-e) Cells in the peripheral blood of WT or Tet2/3 DKO mice were isolated at the indicated time points following pIpC injection and flow cytometric analysis of myeloid (a-c), B-cells (d) and T-cells (e) was performed (n = 7~10 mice per time point examined). Means ± SEM are shown. **P < 0.005, ***P < 0.0005 (Student's t test).

Supplementary Fig. 4

Supplementary Figure 4. Infiltration of livers and lungs of Tet2/3 DKO mice with hematopoietic cells. (a) Enlargement of livers in Tet2/3 DKO mice. Representative photographs of liver from WT and Tet2/3 DKO mice at 4~5 weeks following pIpC injection. Weights of liver at 2~2.5 or 4~5 weeks after pIpC injection were shown at bottom (n = 7~13 per each genotype). Means ± SEM are shown. **P < 0.005, ***P < 0.0005 (Student's t test). (b,c) Hematoxylin and eosin staining of livers at 2~2.5 (b) or 4~5 (c) weeks after pIpC injection. Shown are the loss of normal liver structure and hematopoietic cell infiltration into the livers of Tet2/3 DKO mice. (d) Myeloid cell infiltration into livers of Tet2/3 DKO mice verified by myeloperoxidase staining at 2~2.5 weeks after pIpC injection. (e,f) Histological analysis showing hematopoietic cell infiltration in the lung. Hematoxylin and eosin staining of lungs at 2~2.5 (e) and 4~5 (f) weeks after pIpC injection. For all figures, top panels, 4X magnification; bottom panels, 40X magnification.

Supplementary Fig. 5

Supplementary Figure 5. Histological analysis of bones and spleens. (a,b) Hematoxylin and eosin staining of bones at 2~2.5 (a) or 4~5 (b) weeks after pIpC injection. Note anaemic bones and abnormal morphology of megakaryocytes in Tet2/3 DKO mice. Top panels, 20X magnification; bottom panels, 40X magnification. (c,d) Histological analysis of spleens at 2~2.5 (c) or 4~5 (d) weeks after pIpC injection by hematoxylin and eosin staining. Note disruption of normal splenic structure in Tet2/3 DKO mice. Top panels, 4X magnification; bottom panels, 40X magnification. (e) May-Grünwald-Giemsa-staining of bone marrow aspirates. Note the relatively homogeneous cell population in the DKO sample.

Supplementary Fig. 6

a

b WT DKO

Liver (2.5 week after injection)

104

Mac-1

17.9 0 102

105

53.5 103

104

105

53.2

103 102 0 0 102

103

104

105 104

: CD8a

7.51

103 102 0

75 103

104

CD4

: CD4

104

DK O

o M on

l Ctr

Ctr l

CD8+

105

0.152

4

10

103 102 0

17.2

0 102

103

CD4+

: B220

0.245 105 2.16

4

10

CD8

: CD8a

105

B220+ CD19+

0 102

: B220

***

20 0

102 0

105

B220

3.05

103

*

40

B-

104

: CD19

CD19

: CD19

: CD11b: CD11b 105

***

60

DK O

102 0

10.6 103

DK O

1+

103

Ctr l

0 102

Mac-1+ Gr-1-

104

CD 8+

86.8

Mac-1+ Mac-1+ Gr-1+

DK O

2

28.6

CD 4+ -C on tro l

103 10 0

FSC-A

DK O

Gr-1

104

0

50K 100K 150K 200K 250K

2.6 105 4.22e-3

0

: Gr1

105

FSC-A FSC

ac

0

20 M

0 50K 100K 150K 200K 250K 0

l

0

: Gr1

21.4

50K

**

40

DP

1.01

50K

60

l

100K

DK O

150K

***

Ctr

100K

Percentage

SSC-A

SSC-A

150K

80

Ctr

200K

SSC

200K

***

100

DKO 250K

Percentage

WT 250K

105

92.3 0 102

5.43 103

104

: CD4

105

Supplementary Figure 6. Expansion of myeloid lineage cells and reduction of lymphoid cells in the liver of Tet2/3 DKO mice. (a) Flow cytometry was performed to assess myeloid (Gr-1/Mac-1), B lymphoid (B220+ CD19+) and T lymphoid (CD4/CD8) cell populations in the liver of WT or Tet2/3 DKO mice at 2~2.5 weeks after pIpC injection. Hematopoietic cells were gated as shown in the top panel. Note expansion of FSChi and SSChi cells that normally correspond to myeloid cells in the liver of DKO mice. (b) Summary of the percentage of cell populations shown in a (n = 4 per each genotype). Means ± SEM are shown. *P < 0.05, **P < 0.005, ***P < 0.0005 (Student's t test).

Supplementary Fig. 7 Bone marrow

200K

200K

200K

200K

100K

150K 100K

50K

FSC-A FSC

c

Bone marrow

DKO

Ter-119lo

Ter-119+

CD71+

CD71+

2

0 10

3

10

4

10

B220

: B220

5

10

2.37 2

0 10

3

10

4

10

: B220

5

10

ra

D K O

M on

o

C trl

D K O

n

C

trl

D K O

rl ct b+

G

11 D

3×1037

5 0

B220+

D K O

D K O

o

trl C

M on

n ra G

C trl

***

O

4~5 wk

***

2×1027 1×1017

ce

ll

ct

rl

D K O

rl ct P

D K O

C trl

C D 71 +T er 11 9lo

D K O

***

Te r1 19 +C on tro l

0 0

K D

10

O

102 0

14.6

***

K

102 0

0.86 8.0×10

0.0 0

15

-B

103

KO

103

***

0.46 4.0×10

***

20

D

104

C on tro l-B

Percentage

: CD43

: CD43

104

2~2.5 wk

***

Control-DP DKO-DP

D

: Ter-119

C

C

Ter-119+

Control

D K O

11 b

D

K DKO

Mac-1+ Gr-1-

rl

105

Control

Mac-1+ Gr-1+

ct

104

1.27 1.2×10

10

Mac-1+

ll

103

e

20

105

CD43

105

0 102

0 0

***

30

0

1×1017

ce

Ter-119

: Ter-119

40

2×1027

B

105

***

3×1037

rl

104

Mac-1+ Gr-1-

ct

103

Mac-1+ Gr-1+

D K O

0.112

0

4~5 wk

P

2

10 4.52

0 102

2~2.5 wk

D

0.245

5×1057

D K O

10 103

0 0

C trl

102 0

*

C D 71 +T er 11 9lo

103

104

50

C

on

C

: CD71

104

0.235

0.0306

Erythroid cells in BM (%) Percentage

5

10 21.6

2.02

CD71

B

Ter-119+ Ter-119lo Ter-119+ B220+ CD71+ CD71+ D

: CD71

105

*

D K O

Mac-1+ D

105

: Mac-1 : Mac-1

+

11 b

104

+

18 103

11 b

0 102

l-C

Mac-1

6.01

D

105

D

104

D

103

tro

5.93

0 102

4×1047

4×1047

0 l-C

49.7

***

25

2

10 0

FSC-A FSC

1×1017

***

50

O -C

10

2

50K 100K 150K 200K 250K

3×1037

75

tro

10

3

on

Gr-1

104

3

FSC-A

d

***

100

K

74.1

Percentage

: Gr-1

: Gr-1

42.1105 1.86

104

50K

2×1027

DKO

2.27

FSC-A

100K

0 50K 100K 150K 200K 250K 0

WT DKO

(4~5 weeks after injection)

WT

0 50K 100K 150K 200K 250K 0

0

150K

rl

b

FSC-A

100K 50K

0 50K 100K 150K 200K 250K

150K

ct

FSC-A

0 50K 100K 150K 200K 250K 0

FSC-A

b+

0 50K 100K 150K 200K 250K 0

50K

50K 100K 150K 200K 250K

200K

11

0

FSC-A

D

0

100K

50K

50K

200K

150K

100K

Absolute cell number (X107) in bone marrow

50K

150K

FSC-A

200K

SSC-A

100K

SSC-A

SSC-A

150K

FSC-A

200K

150K

0 50K 100K 150K 200K 250K 250K 0

SSC-A

FSC-A

200K

0 50K 100K 150K 200K 250K 250K 0

0 250K 0

50K 100K 150K 200K 250K

100K 50K

50K

SSC-A

0 50K 100K 150K 200K 250K 250K 0

150K

+G r1 D C + 11 on b+ tro G l -C r1 D + 11 D K b+ O G -C r1 D 11 b+ G r1 -

FSC-A

200K

100K

50K

50K 0 50K 100K 150K 200K 250K 250K 0

150K

Absolute cell number (X107) in bone marrow

100K

SSC

100K

150K

O -C

SSC-A

100K

150K

SSC-A

200K

150K

SSC-A

200K

SSC-A

250K

SSC-A

250K

0

10 0

Blood

250K

250K 0

105

Spleen

250K

WT

Blood

250K

50K

SSC-A

Spleen

250K

SSC

SSC-A

Bone marrow

4~5 weeks after injection

DKO

2~2.5 weeks after injection

Te r1 19 +C on tro l

a

Supplementary Figure 7. Dominance of myeloid cells with reduction of erythroid cells and B cells in the bone marrow of Tet2/3 DKO mice. (a) Expansion of FSChi and SSChi cells in Tet2/3 DKO mice. Relative heterogeneity (WT, top) or homogeneity (DKO, bottom) of cells in bone marrow, spleen and blood, as assessed by separating cells according to their side or forward scattering properties. (b) Representative flow cytometry data assessing myeloid (Gr-1/Mac-1), erythroid (CD71/Ter-119) and B lymphoid (B220/CD43) cell populations in bone marrow of WT or DKO mice at 4~5 weeks after pIpC administration. (c) The frequency of cells shown in b. Means ± SEM are shown. **P < 0.005, ***P < 0.0005 (Student's t test). (d,e) Absolute numbers of myeloid (d) or erythroid and lymphoid (e) cell subsets in bone marrow of WT or DKO mice at 2~2.5 or 4~5 weeks after pIpC injection. Means ± SEM are shown. *P < 0.05, **P < 0.005, ***P < 0.0005 (Student's t test).

Supplementary Fig. 8

b

Spleen (4~5 weeks after injection) DKO 12.9105 1.09

105

2

10

102 0

103 102

42.2

5.87e-3

104 103

0 10

10

4

10

3

0 10

4

10

10

B220+

5

10

: CD4

10

2

CD4+

CD8+

2

2.0×10 8

2.0×10 8

2~2.5 wk

*

1.5

4~5 wk

** 1.5

1.5×10 8

1.5×10 8

1.0×10 8

1

1.0×10 8

0.5

5.0×10 7

*

0.5

5.0×10 7

0

KO

8c trl

D

C

D

D

C

ll

D

ce

B

o

M on

G

ra

n

Mac-1+ Mac-1+ Mac-1+ B220+ CD4+ Gr-1+ Gr-1-

CD8+ D

KO

4c trl

rl ct

KO

DK O

trl C

trl C

DK O

rl ct

DK O

b+ 11 D

rl ct

DK O

DK O

CD8+ CD 8

C

D

8

C D 4

CD4+ CD 4

rl

KO

ct

Gr-1-

B220+ D

B

Mac-1+

B

trl C

o

M on

Gr-1+

DK O

trl C

DK O

DK O

ra

n

Mac-1+ Mac-1+ G

b+

ct

rl

0.0

11 D

*

0

0.0

C

**

1

C

Absolute cell number in spleen (X108)

20

2.46 2

10

CD4

***

30

0

0

5

: CD4

40

102

36.7 96.3 3

***

***

trl

: CD8

104

50

105

4-c

104

CD

103

: B220

0.28 105 1.24

2

c

0 102

CD 4-D KO

B220

20.8

CD8

: CD8

: B220

105

B-D KO

104

B-C

103

Percentage

0 102

0

Mac-1+ Mac-1+ Mac-1+ Gr-1+ Gr-1-

103

0

105

11

104

trl

103

2.06

CD

34.3

104

10 0

105

: CD19

: CD19

CD19

105

20

m on o-C trl

104

8-c

Mac-1

103

: Mac1 : Mac1

m on o-D KO

0 102

5

10

CD

4

10

30

CD 8-D KO

3

10

16.3

trl

5.57 2

0 10

68.7

-c

78.9

102 0

40

trl

0

103

DP

102

50

DP -D KO

103

13.8

104

Percentage

4

10

b-c trl

: Gr1

Gr-1

: Gr1

WT 2.64

105

WT DKO

CD 11 b-D KO

a

Supplementary Figure 8. Expansion of myeloid cells and reduction of lymphoid cells in the spleen of Tet2/3 DKO mice. (a) Representative flow cytometry data assessing myeloid (Gr-1/Mac-1), B lymphoid (B220/CD19) and T lymphoid (CD4/CD8) cell populations in spleens of WT or Tet2/3 DKO mice at 4~5 weeks after pIpC administration. (b) The frequency of cells shown in a. Means ± SEM are shown. *P < 0.05, ***P < 0.0005 (Student's t test). (c) Absolute numbers of myeloid and lymphoid cell subsets in spleens of WT or Tet2/3 DKO mice at 2~2.5 (left) or 4~5 (right) weeks after pIpC injection. Means ± SEM are shown. *P < 0.05, **P < 0.005, ***P < 0.0005 (Student's t test).

Supplementary Fig. 9

b

WT DKO

0

DK O

l ntr co LS k

4 wk

4

4×105

2

2×105

LK k 2w

ntr ol

2 wk

LK -D KO

-C

on

KO

LK D

D KO C on tro l-L K

C on tro l-L SK

0 4w kLK -C o

0

0

LSK

**

6×105

DK O

1

6

l

2

KO

4w

LS k 2w

Number of LK cells (X105)

3

D

K-

C K-

KO

D

*

C on tro l-L in -

2 wk

8

8×105

4

Lin-

DK O

0.0

-L

K l-L C

D

on

3

3.0×104

LK

on

LSK

C

Percentage in bone marrow Percentage of cells

5

tro

KO

l-L

-L

SK

0

SK

20

6

6.0×104

K

***

9

9.0×104

tro

40

1.2×105

l

**

12

tro

60

Number of LSK cells (X104)

80

on

WT DKO 2 weeks after injection

tro

Percentage

- cells Percentage cells among Linwithin ofLin

a

4 wk

Weeks after injection

c

Sorted LSK cells

WT (Tet2+/+ Tet3fl/fl) mice or

or 1st

Tet2-/- Tet3fl/fl ERT2-Cre+ mice

0.75

0.75

0.5

0.5

N.D.

1

1

0.25 0

1  

2  

Tet3

120

0.25 0

1  

Control DKO

Number of colonies / 103 LSK cells

2  

1.25

2  

DKO

1  

Tet2

WT

0

1.25

DKO

2

0.25

DKO

1

DKO N.D.

0.5

0.25 0

Tet3

0.75

0.5

4th

f

After 2nd round of culture

WT

0.75

1

e mRNA levels relative to Gapdh

Tet2

WT

1

3rd

Serial replating in methylcellulose in the presence of 1 μM 4-hydroxytamoxifen

After 1st round of culture

WT

mRNA levels relative to Gapdh

d

2nd

90 60 30 0

1 2 3 4 Number of replatings

Supplementary Figure 9. Altered distribution of hematopoietic stem and progenitor cells upon acute deletion of Tet3 in Tet2-deficient mice. (a) Frequency of LSK (Lin- c-Kit+ Sca1+) and LK (Lin- c-Kit+ Sca1-) cells within Lin- populations (top) or in the total bone marrow (bottom) of WT and Tet2/3 DKO mice at 2 weeks after pIpC injection. Means ± SEM are shown. *P < 0.05, **P < 0.005, ***P < 0.0005 (Student's t test). (b) Absolute numbers of LSK and LK cells in bone marrow of WT and Tet2/3 DKO mice at 2 or 4 weeks after pIpC injection. Means ± SEM are shown. **P < 0.005 (Student's t test). (c) Experimental scheme for colony-forming assay in methylcellulose medium. LSK cells were sorted from bone marrow of WT (Tet3fl/fl) or DKO (Tet2-/- Tet3fl/fl ERT2-Cre+) mice by flow cytometry (n = 4 per each genotype). One thousand cells were serially replated in methylcellulose medium (MethoCult M3534, Stem Cell Technologies) and colonies were counted after 7-9 days. To induce ERT2-Cre recombinase, 1 μM 4-hydroxytamoxifen was added to the cultures. (d,e) Confirmation of Tet2 and Tet3 deletion. Colonies after the first (d) or second (e) round of culture were pooled and quantitative RT-PCR analysis was performed to confirm germline deletion of Tet2 and ERT2-Cre-mediated deletion of Tet3. (f) Combined deficiency of Tet2 and Tet3 leads to increased serial replating capacity in vitro. Colony forming unit assay shows that Tet2/3-deficient, but not WT, LSK cells can be serially replated in methylcellulose medium.

Supplementary Fig. 10

0

75 50 25

2.48

103 2

10 0 3

104

34.8

103

102 0

12.1 3

10 Flt3

104

: c-Kit

51.1

c-Kit

104

100K

4.71e-3

100K

Flt3

103

103

104

CD34 CD34 :

50K 100K 150K 200K 250K

Hoechst Indo-1 (Blue)-ARed

Indo-1 (Blue)-A

*

DKO

103

104

trl -c

D KO

P

P

trl -c

D KO

P

LM

P

ST -D KO

M

D KO

trl

105

: Sca1

105 104

56.3 9.97

103 102 0

32.7 0 102

103

104

: Flt3

105

104 103

LT 27.8

ST 68.9

102 0

105

105

0 102

103

104

: CD34

105

105

104 103

102 0

50 0 102

WT

78.5

102 0 0 102

0 50K 100K 150K 200K 250K0

0.020 0.015 0.010 0.005 0.000

19.3

: Flt3

150K

10

CD48

Side population (%)

0 102

3

4

10 10 CD150

105

104

CD48-CD150+

103 102 0

: CD150

4.44 0 102

103

104

CD34-Flt3- gated

0

2

10 0

105

4

50K

50K 0

103

105

: CD48

0.0134

: Flt3

200K

Hoechst-A

200K

: CD48

Hoechst Blue

250K

LSK 19.4

104

Flt3-/lo gated

250K

ST- Flt3mid Flt3hi HSC (MPP) (LMPP)

105

105

105

DKO

LTHSC

LSK gated

: c-Kit

D KO

ST

-c

trl

D KO

trl -c LT

105

: Flt3

WT

0

DKO

104

10 Sca-1

CD34+ (ST-HSC)

0

105

WT

0 102

150K

104

: Sca1

Ratio of ST-HSC to LT-HSC - WT: 6.517 ± 1.655 - DKO: 4.397 ± 0.756

e

103

: CD34

-c

0 102

105

0 102

CD34(LT-HSC)

Hoechst-A

5

10

LT

4

10

: c-Kit

: c-Kit

100

3

10

CD34 : CD34

f

WT DKO

0

0 10

c-Kit

D KO

-C SC H

d Percentage within LSK Flt3lo/- cells

2

l tro

DKO

on

WT

*

1

1×104

i-C

102 0

2

2×104

Flt 3h

77.7

D KO

20.5

*

3

3×104

trl

ST

-c

102 0

103

LT

id

82.5

4

4×104

ST -D KO

1

1×103

16.4

104

0

105

105

104 103

104

3m

: Flt3

2

2×103

103

: Flt3

Flt

3

0 102

105

ST -C trl

104

105

3×103

0

103

Flt3Flt3 :

*

25

rl

0 102

LMPP

10 0

ct

5

10

**

4

10 0

50

T-

4

10

11.3 2

***

S

3

10

: CD150

10

39.7

2

75

LT -C trl

2

0 10

4×103

Number of LT-HSCs (X103)

LT-HSC

5

10

3

**

LT -D KO

4

10

10

100

trl

3

10

CD150 : CD150

10

10.6

LT -D KO

2

0 10

2.47

3

76.6

Percentage within LSK cells

8.48

10

4

WT DKO

Absolute cell number (X 104)

102 0

9.87

DKO MPP

105

Flt3lo/- gated

102 0

: c-Kit

3

10

49.9

: Flt3

3

10

4

c-Kit

LSK gated

104

CD48

104

105

LSK gated

WT

105

: CD48

105

c

4~5 weeks after injection

DKO : c-Kit

WT : CD48

b

4~5 weeks after injection

Flt3

a

105

: CD150

Supplementary Figure 10. Altered distribution of hematopoietic stem/progenitor cells upon acute deletion of Tet3 in Tet2-deficient mice.

Supplementary Figure 10. Altered distribution of hematopoietic stem/progenitor cells upon acute deletion of Tet3 in Tet2-deficient mice. (a) Acute deletion of Tet3 in Tet2-deficient mice decreases the number of SLAM-marked hematopoietic stem cells (LSK CD150+ CD48-). LSK cells in the bone marrow from WT and DKO mice were analyzed for surface expression of CD48 and CD150. Means ± SEM are shown. **P < 0.005 (Student's t test). (b) LSK cells in bone marrow of WT and Tet2/3 DKO mice were analyzed for surface expression of c-Kit and Flt3, after which the Flt3-/lo fraction was further analyzed based on CD34 expression. CD34- and CD34+ cells in the lower panels represent LT- and ST-HSCs, respectively. (c) Percentage (upper panel) and number (lower panel) of LT-HSCs, ST-HSCs, MPPs and LMPPs in WT and DKO mice. Means ± SEM are shown. *P < 0.05, ***P < 0.0005 (Student's t test). (d) Deficiency of Tet2 and Tet3 results in only a slight decrease in the ratio of ST-HSC to LT-HSCs. (e) Hoechst staining and flow cytometric analysis of the bone marrow of WT and DKO mice. The boxed region in the upper panel indicates the percentage of side population cells, and summary of the results (mean ± SEM) is shown in the lower panel. (f) Increased frequency of CD48+ CD150- population within LT-HSCs (CD34-Flt3- LSK) in DKO compared to WT mice.

Supplementary Fig. 11

b

M C

CMP

D

-C

trl

KO

KO

EP

D

GMP

KO D

0

MEP

c

MEP

d 105

FSC FSC-A

WT

2

0 10

3

10

4

10

CD27 : CD27

5

10

2×1024

0 10

3

10

4

10

5

10

IL-7Ra : IL-7Ra

KO

4~5 wk D

w

k-

C

KO

2~2.5 wk

-4

2

trl

00 D

4.59

102 0

1×1014 trl

103

C

104

w

102 0

105

-2

103

104

: IL-7Ra

k-

103

***

3×1034

LP

50K 100K 150K 200K 250K

105

4.9

104

0 102

5

10

*

Weeks post-injection C

0

4

10

4×1044

LP

0.724

2

3

10

: CD27

Flt3

103

5

10

16

2

10 0

WT DKO

C

FSC-A

104

10 0

2

0 10

50K 100K 150K 200K 250K

: Flt3

0 105

102 0

3

10

Number of CLP cells (X104)

Lin-

: Flt3

3.29

102 0

103

CLP

104

Flt3

103

11.2

104

: Flt3

: Flt3

104

DKO

105

5

10

Lin/CD11c

: Lin/CD11c/7AAD : Lin/CD11c/7AAD

M

G M PC trl

trl

25 trl

O

50

Co

nt ro

l-M

GMP

***

75

DK

O

EP

DK

P

O Co

nt ro l

CMP

Co

nt ro

l-C

M

P

0.00

4~5 wk

-C

0.25

MEP

*

100

KO

**

0.50

GMP

D

0.75

CMP

EP

WT DKO

0

M

: CD34

105

G M PC trl

104

KO

103

D

0 102

D

8.17

1.00

DK

Percentage in bone marrow

CD34 : CD34

105

C

104

P-

103

25

M

0 102

47

CMP

MEP

***

50

C

40.4

102 0

2~2.5 wk ***

75

trl

32.1

-G M

102 0

103

100

C

103

GMP

4

10

Percentage of cells among Lin-

: FcgR

4

10

31.7

LK gated

19.110

10

FcγRII/III

: FcgR

DKO 5

WT DKO

P-

WT 5

Percentage within LK cells Percentage of cells among Lin-

2~2.5 weeks after injection

KO

a

Supplementary Figure 11. Distribution of myeloid and lymphoid progenitors in the bone marrow. (a) Representative flow cytometric analysis of myeloid progenitor cell subsets in the bone marrow of WT and Tet2/3 DKO mice at 2~2.5 weeks after pIpC injection, as assessed by the expression of FcγRII/III and CD34 within LK population (top). Percentage of each myeloid progenitor in bone marrow is shown at bottom. Means ± SEM are shown. **P < 0.005 (Student's t test). (b) Frequency of myeloid progenitor cell subsets within LK populations of WT and Tet2/3 DKO mice at 2~2.5 or 4~5 weeks after pIpC injection. Means ± SEM are shown. *P < 0.05, ***P < 0.0005 (Student's t test). (c) Gating strategy to identify common lymphoid progenitor (CLP) cells in bone marrow. CLPs are defined as Lin- Flt3+ CD27+ IL-7Rα+. (d) Absolute number of CLPs in the bone marrow of WT and Tet2/3 DKO mice at 2~2.5 or 4~5 weeks after pIpC injection. Means ± SEM are shown. *P < 0.05, ***P < 0.0005 (Student's t test).

Supplementary Fig. 12

a

Tet2-/- Tet3fl/fl Mx1-Cre+

WT

or Testers (CD45.2+)

Chimerism 4 wk

WT vs

+

Bone marrow

Blood

200K

200K

200K

SSC-A

SSC-A

250K

SSC-A

250K

150K

150K

150K

100K

100K

100K

50K

50K

50K

0 250K 0

0 50K 100K 150K 200K 250K 250K 0

FSC-A

0 50K 100K 150K 200K 250K 0 250K

FSC-A

200K

SSC

150K

100K

100K

100K

50K

50K 0 0

0 50K 100K 150K 200K 250K 0

FSC FSC-A

FSC-A

SSC-A

150K

150K

50K 100K 150K 200K 250K

200K

SSC-A

200K

SSC-A

Spleen

250K

WT

b

DKO

Competitors (CD45.1+)

DKO

pI-pC i.p.

Recipients (CD45.1+)

50K 0 50K 100K 150K 200K 250K 0

FSC-A

50K 100K 150K 200K 250K

FSC-A

Supplementary Figure 12. Competitive engraftment assay and tumor transfer assay. (a) Experimental scheme for competitive repopulation assay. CD45.2+ bone marrow cells from Tet2+/+ Tet3fl/fl Mx1-Cre- (WT) or Tet2-/- Tet3fl/fl Mx1-Cre+ (DKO) mice were mixed with equal number of CD45.1+ competitor cells and transplanted into lethally irradiated CD45.1+ congenic mice. At 4 weeks after transplantation, chimeric mice were injected with pIpC five times intraperitoneally (week 0) and peripheral blood was examined for donor chimerism at the indicated time. (b) FSChi and SSChi cells in the recipients of WT and DKO splenocytes. Relative heterogeneity (WT, top) or homogeneity (DKO, bottom) of cells in the bone marrow, spleen, blood, as assessed by separating cells according to their side or forward scattering properties.

Supplementary Fig. 13

b

Splenocyte transfer (Tet2fl/fl Tet3fl/fl Mx1-Cre+)

Percent survival

Percent survival

100

c

d

WT DKO

WT

80

150 100 50 0 WT

40

Days post pIpC injection Days post-injection

0 WT

DKO

g

15.9 3.23

0 102

103

104

: Mac1

105

3.91e-3

10

3

10

103

104

27.5105 0.859

4

10

1.77103

2

2

10

0 2

0 10

3

10

4

0

5

10

10

2.41 39.2105 : Ter119

CD71

4

10

0.596

10

1.59 : CD71

5

10

: CD71

4

10

3

10

0.25

0.157 2

0 10

3

10

10

102 0 2

0 10

3

10

4

10

4

Ter-119

: Ter119

0.279

102

5

10

0 102

10 0

18.3 103

104

: Mac1

Mac-1

2

105

9.33 0 102

83.4 103

104

: Mac1

105

102 0 5

Lin

10

43.4

2

10

0 10

102 0 2

3

4

4

10

103 2

10 0

4

10

67.1 0 102

6.09e-3

3

10

102 0 2

10

0 10

3

10

104

CD34

: CD34

4

5

10

: Sca1

10

1.6

4

10

103 102 0

18.1 103

5

10

LK

23.3

5.92105

5

10

4

10

5

5

10 10 Sca-1

: Sca1

3

10

: c-Kit

10

0.488

103

Lin-

48.8

105

84.7 0 102

2.69 103

104

: CD34

105

5

10

1.14

56.1

103

3

10

10 10 27.1 6.73 : Ter119

1.33103

3

4

2

4

0 10

7.3

10

3 4 10 10 c-Kit

105

105

4

3.11 2

10.8 104

10 0

4

10

: c-Kit

102

103

2

0 10

1.42

: Mac1

103

105

103

0 102

4

10

5

10

0

Spleen

: CD71

: CD71

2.59

Bone marrow

WT 5

103 10 0

104

104

105

: Gr1

DKO

103

: Mac1

25.6 105 0

0

4

10

Gr-1

: Gr1

: Mac1

105

0 102

13.20 87.8

74.8 0 102

105

94.9

11.9 105 7.78e-3

4

102 0

102 0

: Lin

44.6

WT DKO : Gr1

WT DKO

102 0

103

DKO

105

: c-Kit

WT

3

10

104

Bone marrow

0

DKO

104

WT 1.83

: FcgR

WT

39.5 105 1.95e-3

Spleen

0

0.5

0

Blood

0.2

1

5

10

Spleen

DKO : Gr1

0.4

1.5

: Gr1

0.6

WT

***

2

Liver weight (g)

0.8

DKO

i

: Gr1

***

DKO

WT

h

Spleen weight (g)

f

50

: Lin

30

c-Kit

20

100

: c-Kit

10

e

*

FcgRII/III

0

150

LK gated

20

DKO

Lin- gated

Neutrophils /μl (X103)

DKO

: FcgR

40

10

DKO

WT

60

0

j

***

200

WBCs /μl (X103)

a

0.149 2

0 10

3

10

4

10

: Ter119

5

10

Supplementary Figure 13. Transfer of splenocytes from Tet2/3 DKO mice leads to myeloid leukemia in secondary recipients.

Supplementary Figure 13. Transfer of splenocytes from Tet2/3 DKO mice leads to myeloid leukemia in secondary recipients. (a) Kaplan-Meier curve representing the percent survival of recipient mice transplanted with 2 x 106 splenocytes from WT (Tet2fl/fl Tet3fl/fl) and diseased Tet2/3 DKO (Tet2fl/fl Tet3fl/fl Mx1-Cre+) mice (n = 10 per each group). (b) May-Grünwald-Giemsa-stained peripheral blood smears of recipient mice. (c) Recipients of Tet2/3 DKO splenocytes developed progressive leukocytosis with neutrophilia. Means ± SEM are shown. *P < 0.05, ***P < 0.0005 (Student's t test). For a summary of other hematopoietic parameters, see Supplementary Table 2b. (d) Enlargement of spleens of mice that received Tet2/3 DKO splenocytes. (e) Representative photographs of femurs and tibiae from recipients of WT or Tet2/3 DKO splenocytes. (f) Weights of spleen or liver. Means ± SEM are shown. ***P < 0.0005 (Student's t test). (g) Hematoxylin and eosin staining of livers show loss of normal liver structure and infiltration with hematopoietic cells. 4X magnification. (h) A representative flow cytometric analysis of myeloid-lineage cells (Gr-1+/Mac-1+) in the bone marrow, spleen and blood of recipient mice. (i) Increase in the frequency of Lin- populations in the spleen from recipients of Tet2/3 DKO splenocytes. (j) A representative flow cytometric analysis of erythroid-lineage cells (Ter-119+/CD71+) in the bone marrow and spleen of recipient mice.

Supplementary Fig. 14

10

20

30

40

3

10

102 0

51.8

1

0 10

2

3

10

4

g

105

10

3.25

103

72.2 0 102

103

104

i

103

67.9 104

Mac-1

0.584

7.83

103 2

10 0

103 102 0

0.191

1.54 0 10

3

10

4

10

2.68

10

4

10

103

103

104

: Ter119

30.9105 15.3

CD71

1.87

0 102

5

: Ter119

12.2

10 0

1.11

102 0

0.723 0 102

103

104

105

Ter-119 : Ter119

103 102 0

105

60

4.98 103

104

: Mac1

105

* ***

20

91.1 100

4

10

103

105

*

40

0

52.4 0 102

102 0

***

25

4.71 0 102

4.12 103

104

: Mac1

105

***

75 50

***

25 0

105

4

103

104

***

50

15.4

10

7.06

2

10

41.4

***

75

0

5

10

100

Bone marrow

9.67

4

10

10

4

DKO

Spleen

10

2

: CD71

: CD71

4

105

DKO 26.8105 0.972

1.17

: CD71

: CD71

WT 5

0 10

3

: Mac1

5.61 103

: Mac1

10

2.12 2

10

: Gr1

Gr-1

: Gr1

10

0 102

15.6

24.6105 0.0563

1.88

4

102 0

102 0

13

: Mac1

105

10

11.6105 1.27

104

102 0

3

5

: Mac1

WT DKO

104

3.7

2

0

WT DKO

104

78.4

Spleen

0.5

WT

DKO : Gr1

1

20 0

43105 3.88

1.46

e

***

Blood

2  

1.5

105

: Gr1

1  

2

WT

: Gr1

0.4 0.3 0.2 0.1 0

h

***

: Gr1

***

Liver weight (g)

f

Spleen weight (g)

Days post-injection

80 60 40

DKO

W TM ac 1+ D K O -M ac 1+ W TTe r1 19 D K + O -T er 11 9+ W TC D 19 D + K O -C D 19 W + TC D 4/ D C K D O 8 -C D 4/ C D 8

0

WT

W TM ac 1+ D K O -M ac 1+ W TC D 4/ C D 8 D K O -C D 4/ C D 8 W TC D 19 + D K O -C D 19 +

0

Neutrophils /μl (X103)

25

***

W TM ac 1+ D K O -M ac 1+ W TTe r1 19 D K + O -T er 11 9+ W TC D 19 D + K O -C D 19 W + TC D 4/ D C K D O 8 -C D 4/ C D 8

DKO

100 75 50 25 0

Percentage (bone marrow)

50

WT DKO

Percentage (spleen)

75

d

Percentage (blood)

WT

c

Bone marrow

100

Percent survival

b

Bone marrow transfer (Tet2fl/fl Tet3fl/fl ERT2-Cre+)

WBCs /μl (X103)

a

0.0838 0 102

103

104

: Ter119

105

Supplementary Figure 14. Transfer of bone marrow cells from Tet2/3 DKO mice leads to myeloid leukemia in secondary recipients.

Supplementary Figure 14. Transfer of bone marrow cells from Tet2/3 DKO mice leads to myeloid leukemia in secondary recipients. (a) Kaplan-Meier curve representing the percent survival of recipient mice transplanted with 2 x 106 nucleated bone marrow cells from WT (Tet2fl/fl Tet3fl/fl) and diseased Tet2/3 DKO (Tet2fl/fl Tet3fl/fl ERT2-Cre+) mice (n = 5 per each group). (b) May-Grünwald-Giemsa-stained peripheral blood smears of recipient mice. (c) Recipients of Tet2/3 DKO bone marrow cells developed progressive leukocytosis with neutrophilia. Means ± SEM are shown. ***P < 0.0005 (Student's t test). For a summary of other hematopoietic parameters, see Supplementary Table 2c (d) Enlargement of spleens of mice that received Tet2/3 DKO bone marrow cells. (e) Representative photographs of femurs and tibiae from recipients of WT or Tet2/3 DKO bone marrow cells. (f) Weights of spleen or liver. Means ± SEM are shown. ***P < 0.0005 (Student's t test). (g) Hematoxylin and eosin staining of livers show loss of normal liver structure and infiltration with hematopoietic cells. 4X magnification. (h) A representative flow cytometric analysis of myeloid-lineage cells (Gr-1+/Mac-1+) in the bone marrow, spleen and blood of recipient mice. Summary of the percentage of each cell population is also shown in the right panel. (i) A representative flow cytometric analysis of erythroid-lineage cells (Ter-119+/CD71+) in the bone marrow and spleen of recipient mice.

Supplementary Fig. 15

WT

40

0

20

40

Days post-injection

0.1 0

1  

1 0.5 0

2  

WT DKO

1

0.357

3

10

55.2 0 102

2

WT DKO

g

50 0

30 105 0.0442

104

102 0

100

3.25

104 3

10

102 0

14.4 4.93 103

104

WT

105

0 102

103

104

105

: Mac1 : Mac1 105

0.0668

5.06 105 0.1

4

10

103 102 0

86.7 0 102

4.49

4

10

103

104

105

*** 100

***

75

***

50 25 0

100

***

***

75

***

50 25 0

102 0

8.18 27.2 103

DKO

91.8

Spleen

0.2

1.5

105

e

***

DKO : Gr1

0.3

2

WT

: Gr1

Liver weight (g)

0.4

h

**

: Gr1

2.5

***

: Gr1

0.5

Spleen seight (g)

f

150

0 102

W TM ac 1+ D K O -M ac 1+ W TTe r1 19 D K + O -T er 11 9+ W TC D 19 D + K O -C D 19 W + TC D 4/ D C K D O 8 -C D 4/ C D 8

0

Neutrophils /μl (X103)

DKO

20

DKO

W TM ac 1+ D K O -M ac 1+ W TTe r1 19 D K + O -T er 11 9+ W TC D 19 D + K O -C D 19 W + TC D 4/ D C K D O 8 -C D 4/ C D 8

60

Percentage (bone marrow)

Percent survival

WT DKO

80

200 150 100 50 0

d

***

Percentage (spleen)

WT

100

c

Bone marrow

b

Mac-1+ cell transfer (Tet2fl/fl Tet3fl/fl Mx1-Cre+)

WBCs /μl (X103)

a

68.2 103

104

105

: CD71

33.5 105

10

0.259

0.0802

10

10

102 0

1.35

103 102 0

0.533 0 102

103

104

105

0.326Ter119 18.9105 :

CD71 104

0.284 0 102

103

104

102 0 103

104

2.12

103 102 0

105

Ter-119

: Ter119

104

105

0 D K O -M ac 1+ TC D 4/ C D 8 D K O -C D 4/ C D 8 W TC D 19 + D K O -C D 19 +

103

W

0 102

1+

105

ac

104

25

M

103

Mac-1

82.3

T-

10 0

13.7 7.2

50

W

2

***

105

104

1.3 0 102

72.2

10

***

75

1.56 Ter119 5.2 :

2.61

103

10 0

3

: Mac1 : Mac1

4

4.78

3

105

: CD71

2.41

4

2

0 102

DKO

: CD71

: CD71

105

10

104

Bone marrow

WT

3

***

100

Spleen

i

104

9.61

Percentage (blood)

14.1 105 0.89

Blood

0.0186

: Gr1

105

Gr-1

: Gr1

: Mac1 : Mac1

0.804 0 102

103

104

: Ter119

105

Supplementary Figure 15. Transfer of Mac-1+ cells from Tet2/3 DKO mice leads to myeloid leukemia in secondary recipients.

Supplementary Figure 15. Transfer of Mac-1+ cells from Tet2/3 DKO mice leads to myeloid leukemia in secondary recipients. (a) Kaplan-Meier curve representing the percent survival of recipient mice transplanted with 2 x 106 Mac-1+ cells from WT (Tet2fl/fl Tet3fl/fl) and diseased Tet2/3 DKO (Tet2fl/fl Tet3fl/fl Mx1-Cre+) mice (n = 9 per each group). (b) May-Grünwald-Giemsa-stained peripheral blood smears of recipient mice. (c) Recipients of Tet2/3 DKO Mac-1+ cells developed progressive leukocytosis with neutrophilia. Means ± SEM are shown. ***P < 0.0005 (Student's t test). For a summary of other hematopoietic parameters, see Supplementary Table 2d. (d) Enlargement of spleens of mice that received Tet2/3 DKO Mac-1+ cells. (e) Representative photographs of femurs and tibiae from recipients of WT or Tet2/3 DKO Mac-1+ cells. (f) Weights of spleen or liver. Means ± SEM are shown. ***P < 0.0005 (Student's t test). (g) Hematoxylin and eosin staining of livers show loss of normal liver structure and infiltration with hematopoietic cells. 4X magnification. (h) A representative flow cytometric analysis of myeloid-lineage cells (Gr-1+/Mac-1+) in the bone marrow, spleen and blood of recipient mice. Summary of the percentage of each cell population is also shown in the right panel. (i) A representative flow cytometric analysis of erythroid-lineage cells (Ter-119+/CD71+) in the bone marrow and spleen of recipient mice.

Supplementary Fig. 16 4 3 2 1 0

NES: -5.467 FDR < 0.0001 P < 0.0001

-0.1 -0.2 -0.3

12

Color Key and Histogram

Pre-MegE

NES: 9.382 0 FDR < 0.0001 P < 0.0001 -0.1

DE genes in LSK_DKO Vs LSK_Ctrtl

NES: -8.58 FDR < 0.0001 P < 0.0001

-0.2

-0.2

-0.3

Color Key

Color Key

(Ivanova et al., Science, 2002)

8

CLP 0 -0.1

NES: -2.34 FDR < 0.0001 P < 0.0001

(Sanjuan-Pla et al., Nature, 2013)

4

Meis1 Gata2 Nap1l3 Rarb Klf12 Prdm16 Hoxa5 Lmo2 Zfp37

Genes

Irf6

Color Key

Mycn Hlf Msi2 Hoxa9

−1

0

1

Row Z−Score

Runx1t1

LSK_DKO_B

Zfp532

LSK_DKO_A

LSK_Ctrtl_A

Mecom

LSK_Ctrtl_B

Zfp612

Ndn

-1

0

LSK_Ctrtl_A

Z-score

1

LSK_DKO_B

Z Scores of RPKM values

Z Scores of RPKM values

LSK_DKO_A

HSC-specific genes (Riddle et al., Cell, 2014)

LSK_Ctrtl_B

LSK_DKO_A

LSK_Ctr tl_A

Tcf15

Early progenitors (s-mpp)

Nr3c2

Epb4.1l3 Mecom Gabbr1 Il17re Nkx2−3 Hoxa9 Msi2 Hlf Stxbp4 Phxr4 Padi4 Hnf4a Eya1 Prkd2 Tanc2 Tcf7l2 Nfatc2 Prkce Zfp287 BC031353 Nlgn2 Arhgef5 Dab2ip Rnf122 Nrgn Pglyrp2 Itih5 Gcnt2 Fam69b Socs5 Meis1 Rbpms Zfp608 Ddx58 Sfi1 2900026A02Rik Vezf1 Tnfsf10 Dnmt3b Nfkbiz Gramd1a Oas2 Csad Alcam Arrdc3 Ctla2b Cand2 Ppp1r13b Fchsd2 Hmga2 Samd9l Cxxc5 Zfhx3 Impact Pde4b Ifi44 Chd3 Trp53inp1 Abcg1 Tmbim4 S100a10 Ffar2 Ly6a Tmem176a Atg7 Dnase2a Oas1a Ifitm3 Ifitm1

(Ng et al., Immunity 2009)

Color Key

−1

0

1

Row Z−Score

Z Scores of RPKM values

Color Key

−1

0

1

Row Z−Score

Z Scores of RPKM values

Rhd Bex4 Nckap1 Slc40a1 Pla2g4c Igf2r Trib2 Ermap Dmd Gata1 Shank3 Lphn2 Arhgef12 Car2 Abcb4 Rab4a Grb10 Ppp1r9a Mtap7 Tnik Aqp9 Hemgn Mllt3 Gnb4 Sorbs1 Nfia Slc12a2 Car1 Slc22a3 Casc4 Vamp5 Tgfbr3 Aldh7a1 Mast4 Xrcc5 Tal1 9830001H06Rik Mta3 Lpin2 Igf1r Ssbp3 Cd81 Tspan32 Foxn3 Creg1 Snap23 Cd97 Apoe St8sia6 Mt1 Scin

(Ng et al., Immunity 2009)

Z Scores of RPKM values

Supplementary Figure 16. Tet2 and Tet3 differentially modulate stem cell- and lineage-affiliated transcriptional programs. Z Scores of RPKM values

Papss2 Cybb Cx3cr1 Csf1r Igsf6 C3 Pld4 Pmaip1 Sema4a Ms4a3 Tifab Clec7a Ccl6 Mtus1 Hdc Emr1 Pik3r6 Kmo Lgals3 Cldn15 Nr p1 Fcgr3 Ptpro Alas1 Dmkn Lpxn Csf2rb2 5430435G22Rik Sepx1 Ap3s1 Idh1 Fcgr2b Trem3 1190002H23Rik Dram1 Cfp C1galt1c1 Ctsz Tmem38b Plod3 Psap Lta4h Ccbl2 Csf2rb Acot9 Mlkl Mapkapk3 Sorl1 Nucb2 Sdf2l1 Kctd20 Lamp2 2010111I01Rik H47 Sh2b2 Cd48 Erlin1 Mtm1 Gng12 Edem1 Ostf1 Fabp5 Zeb2 2810417H13Rik Nnt Dpp4 Ube2w Actr3 Wdr1 Sgpl1 Idh2 Sgk3 5430427O19Rik Hsp90b1 Itpr1 Pde4d

Genes

Rbpms

Genes

Egr1

Genes

Hoxb3

LSK_DKO_B

Igf2bp2

LSK_DKO_B

Pbx1

LSK_DKO_B

Prdm5

LSK_DKO_A

Nfix

LSK_DKO_A

Zfp521

HSC-specific genes (stem)

Zfp467

Csf1r Csf2rb Csf2rb2 Csf3r Itgam Ly6c2 Mpo Irf8 Sfpi1 Mnda Ifi205 CD14 Fcgr2b Ncf1 Ncf2 Ncf4 Ctsg Lyz1 Lyz2 Tcf3c Dntt Satb1 Notch1 Sox2 CD72 Ets1

LSK_DKO_A

Glis2

Mnda Cd14 Ccr2 Csf1r Slfn2 Mpo Tyrobp Ctsg Ms4a6c Prtn3 Ctsh Gria3 Lyz2 Ccl9 Rassf4 Irf8 Plac8 Lyz1 Mgst1 Csf2rb2 Ahnak 4632428N05Rik Scpep1 H2−DMb2 Tgfbi S1pr3 Ms4a6b Fcer1g Anxa2 Idh1 Tcn2 Ctss Fcgr2b Tcfec Unc93b1 Anxa1 Ifi205 Grn Naga Ap1s2 Hfe Cst3 Ms4a4b Soat1 Napsa BC064078 Ugt1a7c Asah1 BC013712 Tnfaip8l2 Gatm Arhgap26 Cd52 Ly6e S100a6 Ralb Gm885 Myo1f Tubb6 Emb Lta4h Hvcn1 Gpr160 Atp8b4 1600014C10Rik Sla Rab3d H2−DMb1 Tmem50b Mgst2 Mapkapk3 Serpinb1a Sell Cotl1 Tax1bp3 Sorl1 Fgl2 Rab32 0610031J06Rik Twf2 Gramd3 Arpc1b Slc29a3 Cd300a Tmsb4x Lbp Lst1 Plxnb2 Rps6ka1 Hexa Anxa6 Coro1a Litaf Ceacam1 Rab44 Ncf4 Sfpi1 Diap2 Glipr1 Tpm4 Il6st Spns3 Abcd1 Pgam1 Hk3 Trf Fgd2 Fes Cnn2 Cd68 Arhgdib Cd53 Man2b1 Pkm2 Ncf2 Serpinf1 Lass6 S100a11 Vim Alox5ap Rac2 Itgb7 Dhrs7 Ncf1 Pold4 Hk2 Laptm5 Edem2 Myo1g Bex6 Rab31 Lcp1 Tmem173 H2−M3 Sirpa Tnfrsf1a Rin3 Sh3bgrl3 Tmem176a Gpi1 Hpcal1 Rgs19 H2−DMa Gbp3 Ptpn6 Fcgrt Ffar2 Vwa5a Krtcap2 Lsp1 Gm2a Ninj1 Lrrc33 Myadm Rpl13 Tmem205 Parp8 Lpcat2 Arpc2 Flnb Acpl2 Ivd Ifi47 Skap2 Dpp4 Ube2w Tpd52 Pak1 Scamp2 Kctd12 Hexb Csf3r Fam107b Fam102b Msra Myl12b Psmb8 Psmb10 Swap70 Ramp1 Plin3 Sypl Parl Prkcd Idh2 Lpar6 St8sia4 A630001G21Rik Fxyd5 Wls Tmem176b 1810058I24Rik Map3k1 Arl6ip1 Akap13 Ptpre Sh2d5 Macf1 Smad5 Elmo1 Trp53bp1 Gabpb1 Slco3a1 Znrf1 Arid1b Sesn1 Gnaq Map4k4 Cdk19 Mast3 H2−Ob Atp2b4 Camk2d Tsc22d1 1110028C15Rik Satb1 Hmga2 Wdfy1 Fmnl2 Notch1 Adamts10 AI504432 Eltd1 Camk2g Sox4 Pag1 Xpo7 Marcks Anks1 Alcam Lonrf3 9030619P08Rik 4931406C07Rik Nfkbiz Aff3 Dusp2 Ets1 Nfkbid Snn Calcrl Epb4.1l4b Arl4c Cd72 Ttpa P2ry14 Fam134b Repin1 Tmprss3 Gpsm1 Ccnd1 Hdgfrp3 Esr1 Jakmip1 AW555464 Dntt Il18r1

LSK_Ctrtl_B

Hoxb4

DKO

1

LSK_Ctrtl_B

Etv6

0

LSK_Ctrtl_B

Runx1

WT −1

Row Z−Score

LSK_Ctrtl_A

Ndn Dsg2 2510009E07Rik Prkaa2 Zfp532 Fhl1 Mecom Crim1 Cuedc1 Nbea Gucy1a3 Cdkn1c Bgn Msi2 Sdpr Pf4 Hlf Cadps2 Cdk14 Mylk Fgd5 Chrnb1 Dip2c Hoxa10 Mycn Crispld1 Fnbp1l Mllt4 Gkap1 Ppp1r9a Gimap8 Hdgfrp3 Mmrn1 Asah2 Angpt1 Prdm16 Zbtb4 Gimap1 Nrxn1 Per3 Pear1 Itsn1 Pglyrp2 Mamdc2 Nfat5 Armcx1 Rhobtb3 Gata2 Trove2 Parp12 Csgalnact1 Meis1 Mpzl1 Inadl Dst Smarca2 Psd3 Serpinb9 Spns2 Med12l Egr1 Gimap5 Rgs1 Dach1 Maml2 Pdzk1ip1 Lass4 Atp10d Utrn Pbx1 6720401G13Rik Osbpl1a Igf1r Ocrl Diap1 Ikzf2 Sgms1 Rbbp6 Ppp1r15a Akap13 Sord P2rx1 Stat1 Ubl7 S100a1 Ptgs1 Selp

Vdr

Hoxb5

d

DKO

1

LSK_Ctrtl_A

0

Row Z−Score

LSK_Ctrtl_A

WT −1

Genes

DKO

Lymphoid and myeloid genes primed in HSCs (s-myly)

WT

Row Z−Score

Genes

−1.5 −0.5 0.5 1.5

GMP-specific Erythroid genes primed in HSC (s-ery) Genes (d-my)

c

0

b

LSK_DKO_B

Count

Pre-GM

HSC 0

LSK_Ctr tl_B

Enrichment score

a

Supplementary Figure 16. Tet2 and Tet3 differentially modulate stem cell- and lineage-affiliated transcriptional programs. a, Gene set enrichment analysis (GSEA) of RNA-Seq data shows that the pre-granulocyte/ macrophage progenitor (pre-GM) gene signature is significantly enriched for genes up-regulated in Tet2/3 DKO compared with WT LSK cells, whereas the HSC, pre-megakaryocyte/ erythrocyte progenitor (Pre-MegE) and common lymphoid progenitor (CLP) gene signatures are enriched in genes downregulated in Tet2/3 DKO compared with WT LSK cells. b-d, Heatmap representation showing differential expression of genes highly expressed in HSC and their immediate downstream progenitors (b, c), as well as lineage-affiliated genes (d) in Tet2/3 DKO LSK cells compared with WT LSK cells. The gene sets (including stem, s-mpp, s-ery, d-my and s-myly) have been described. Only genes with a p-value ≤ 0.05 and fold change > 1.5 or < 0.67 were considered. Asterisks in b indicate genes used to induce reprogramming of differentiated hematopoietic cells into induced HSCs. The color key for all heatmaps indicates row-wise scaled RPKM values (z-score).

Supplementary Fig. 17

All 0.6 Frequency

Fraction of CpGs

d

CpGs covered ≥ 10X (n = 8,244,600)

0.8

0.4

0.2

1

0.2

0.8

0.15

0.6

0.1

0.4

0.05

0.2 0

0

0

Hypermethylated

b

Frequency

%(5mC + 5hmC)/ total C

CpGs covered ≥ 20X (n = 422,570)

0.2

0.8

0.15

0.6

0.1

0.4

0.05

0.2 0

0

Frequency

% methylation in DKO

Hypomethylated 1

0.2

0.8

0.15

0.6

0.1

0.4

0.05

0.2 0

c

0 Genome

% methylation in WT

Random genome fragments

All genes

% 5mC + % 5hmC

1

DMRs

a

100

100

80

80

60

60

40

40 WT

20

WT 20

DKO

0

0 TSS -2 kb

DKO

TTS Gene body

-40 + 2 kb

-20

0

20

40

Relative position in random genome fragments

Supplementary Figure 17. Loss of Tet2 and Tet3 results in aberrant gene expression and DNA methylation.

Supplementary Figure 17. Loss of Tet2 and Tet3 results in aberrant gene expression and DNA methylation. a, Histogram of genome-wide CpG modification (5mC + 5hmC) in WT (blue) and Tet2/3 DKO (red) LSK cells at CpGs covered by at least ten reads. The histogram shows a typical bimodal distribution where the majority of CpGs are highly methylated. b, Scatter plot of genome-wide CpG methylation comparing WT LSK (x-axis) and Tet2/3 DKO LSK (y-axis) cells at individual CpGs (black dots) covered by at least 20 reads in each condition. The graph indicates the genome-wide increase of DNA methylation in Tet2/3 DKO LSK cells, and the Lowess curve confirms that the majority of CpGs in both WT and DKO genomes are methylated. c, Left, Average DNA methylation (5mC+5hmC) along gene regions, including 2 kb upstream of the transcription start sites (TSS) and 2 kb downstream of the transcription termination sites (TTS). Considering all genes, the average level of DNA methylation is slightly but consistently increased in Tet2/3 DKO LSK samples (red lines) compared to the control LSK samples (blue lines); note the close correlation between the triplicate biological samples in each case. Similar results were obtained when considering upregulated or downregulated genes (see Figure 5d). Right, Average DNA methylation (5mC+5hmC) in randomly chosen genome fragments of similar size. d, DMRs are significantly enriched in promoters and exons.

Supplementary Fig. 18

a

CGI shores 12005 171 (1.42%) 3 7 1539 116 135 53 (0.44%) 5

Downregulated

3

No. of CGI shores less methylated in DKO Upregulated Downregulated

224 20 16

Total no. of canyons

1,135

- Downregulated

- Downregulated

67

No. of canyons that expand in DKO

4

- Downregulated

3

Genes associated with shrinkingLSK_DKO canyons Vs LSK_Ctrtl(n=525) 10

LSK_DKO Up Regulation −−−−>

5 0

●

● ●

●

● ●

● ●

●

●

●

● ●

●

●

●

●

●

● ●

●

● ●

WT

5

●

DKO

●

●

● ●

●

0

● ●

Car2

-5

Gcnt2

67

WT

-5

67

3

●

-5 −5

0 0

5 5

10

Mean of Normalized Counts

10

15 15

Mean of normalized counts

-5

0

5

33.26%

19.46%

17.79%

0.2073

10

15

Downregulated genes with shrinking canyons 50

●

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●

19

20

e

4

●

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● ●● ● ● ●● ● ●● ● ● ● ● ●● ●● ● ● ● ● ● ● ● ● ●● ● ● ●● ● ● ● ● ● ● ● ● ● ● ●● ●●● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ●● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ●● ● ●● ● ●● ● ● ● ●● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ●● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ●● ● ● ●● ●● ● ● ● ● ● ● ● ● ● ●● ● ● ● ● ● ● ● ●● ● ● ● ● ●● ● ● ●● ● ● ● ● ● ● ● ●● ● ● ● ● ● ● ● ● ● ● ● ● ● ●●● ● ● ● ●● ● ● ● ● ● ● ● ● ●● ● ● ● ● ● ●● ● ● ● ●● ● ● ● ● ● ● ●● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ●● ●●● ●●● ● ● ● ● ● ● ●●● ● ● ● ●● ● ● ● ● ●● ● ● ● ●● ● ● ● ● ● ● ● ●●●● ● ● ● ● ● ● ●● ●● ● ● ● ● ● ● ● ● ● ● ●● ● ● ● ● ● ● ● ●● ● ● ● ●●● ● ● ● ● ● ● ●● ● ●● ● ● ● ● ● ● ● ● ● ● ● ●●● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ●● ● ●● ●●● ● ● ● ●● ●● ● ● ● ● ● ● ●● ●● ● ● ● ● ● ● ● ● ● ●●● ● ● ● ● ● ● ● ●●● ● ●● ● ● ●● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ●● ●●● ● ● ● ● ● ● ● ● ● ● ● ● ● ●● ● ● ●●● ● ● ● ● ●● ● ● ●● ●● ●● ● ● ● ● ● ● ● ●● ● ● ● ●● ● ●● ● ●● ● ● ● ● ● ●●● ● ● ● ● ● ● ● ● ●● ●● ● ● ● ● ● ●● ● ● ● ●● ● ● ● ●● ● ● ● ● ● ● ●● ● ● ● ● ● ● ● ● ● ●● ● ● ● ● ●● ● ● ● ● ●● ● ●● ● ● ● ● ● ● ● ● ●● ● ● ● ● ● ● ●● ● ● ●● ●● ● ● ●● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ●● ● ● ● ●● ● ●● ●● ●●● ● ● ● ● ● ●● ●● ●● ● ●● ●● ● ●● ● ● ● ●● ● ●●●● ● ● ●● ● ●● ● ●● ● ● ● ● ● ● ● ● ● ●● ● ● ● ● ● ●●●● ● ● ● ● ● ● ● ● ● ● ● ●● ● ● ● ● ● ● ● ● ●● ●● ● ● ● ●● ●●● ● ●● ● ● ● ●● ● ● ● ● ● ●●● ● ● ● ● ●● ● ● ●● ●● ●● ● ● ● ● ● ● ● ● ●● ●● ● ●● ● ● ● ●● ● ● ●●●●● ● ● ●● ● ● ●● ● ● ●●●● ● ● ● ● ● ●● ●● ● ● ● ● ● ● ● ●●●●● ● ●● ● ● ● ● ● ● ●●● ● ● ● ● ● ● ● ● ● ●● ● ●●● ● ● ●● ● ● ● ● ● ● ● ● ●● ● ● ● ● ● ● ●●● ● ● ● ● ● ● ● ●● ● ● ● ●● ● ●● ● ●● ● ● ● ● ●● ● ● ●●● ● ●● ● ● ● ●● ●● ● ●● ●●● ●● ● ● ● ● ●● ● ● ● ● ●● ● ●● ● ● ● ● ●● ● ● ● ● ●● ● ● ● ● ● ●● ●● ● ● ●● ● ● ●● ● ● ● ● ●●● ● ● ●● ● ● ● ● ●●● ● ● ● ● ● ● ●● ● ● ● ● ● ● ● ● ● ● ● ●●● ● ● ●● ● ● ● ●●● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ● ●● ●●● ●● ●● ● ●●● ● ● ● ● ● ●● ● ● ● ● ●●● ● ● ● ●● ●● ● ●● ● ● ●● ● ● ● ●● ●● ●●● ●● ●●● ●● ●● ● ●● ● ● ●●● ● ●● ● ●●●● ● ● ● ● ● ● ● ● ● ● ● ● ●●● ● ● ●●●● ● ● ● ● ● ●● ● ● ● ● ● ● ● ● ● ● ● ●● ● ● ●● ● ● ● ● ● ●● ●● ● ● ●● ●●● ● ● ● ● ● ●● ● ● ● ●●● ● ● ● ● ●● ● ● ● ● ●●● ● ● ● ●● ●●●● ● ● ●● ● ● ● ●● ● ● ● ● ●● ● ● ● ● ● ● ● ● ● ● ●● ●●●● ● ● ● ● ● ●● ● ● ●●● ● ● ●● ● ●● ● ● ● ●● ●● ● ● ● ●● ● ●● ● ●● ● ● ● ●● ● ●● ●● ●● ● ● ● ● ● ● ● ● ● ●●●● ● ● ● ● ● ● ●● ● ● ● ● ● ●● ● ● ● ● ● ● ● ● ● ● ● ● ●● ● ● ●●● ● ● ● ●● ● ● ● ● ● ●● ● ● ● ● ● ● ● ● ●● ●● ● ● ● ● ● ● ● ● ● ● ●● ● ● ● ● ● ● ● ●● ● ● ● ● ●● ● ● ●● ●● ● ● ● ● ● ● ● ● ●● ● ● ● ● ● ● ● ●● ● ● ● ● ●● ●● ● ●● ●● ● ●● ● ● ● ● ● ● ● ●● ● ●● ● ● ● ● ● ● ● ● ● ●● ● ● ● ● ● ● ● ● ● ● ● ●● ●● ● ● ● ● ●

Genes associated with expanded canyons (n=70)

●

● ●

● ● ● ●

●

●

3.838e−31

29.8%

0 is canyon center

●

● ●

● ●

●

−5

Log2FoldChange(LSK−DKO/LSK−Ctrl)

● ● ● ● ●

0 )

70

- Upregulated

20

100

59 (5.20%)

Genes associated with expanded canyons

0

100

525 19

10

c

77

- Upregulated

-20

Methylation difference (DKO-WT)

465 (40.97%)

Genes associated with canyons that shrink

1539

-40

28

No. of canyons that shrink in DKO

d

224

846 (74.54%)

- Upregulated

135

-5

% 5mC + %5hmC % Methylation (5mC + 5hmC)

No. of canyons close to a gene

16

0

0

b

116

80

Downregulated No. of CGIs less methylated in DKO Upregulated

20

60

No. of CGI shores more methylated in DKO Upregulated

5

40

Downregulated

Differentially expressed genes

20

No. of CGIs more methylated in DKO Upregulated

Log2 fold change (DKO LSK/control LSK)

Total no. of promoter CpG islands (CGIs)

0 100 0

Mean of normalized counts

WT DKO

DKO

0 10 0 100 0 100 0

Supplementary Figure 18. DNA methylation at CpG islands and CGI shores and differentially methylated regions (DMRs).

WGBS

WT

Gcnt2

RNA-seq

10

Supplementary Figure 18. DNA methylation at CpG islands and CGI shores and differentially methylated regions (DMRs). a, Left panel, Summary of the number of CpG Islands (CGIs) and CGI shores within or at the promoter regions (± 2 kb) of genes that show altered methylation in WT compared to Tet2/3 DKO LSK cells. Right panel, lack of a clear relation between the DNA modification change in CGI shores at promoters (n=12,005) and the change in expression level of the associated genes. The left, central and right sets of dots show CGI shores with decreased, unchanged or increased methylation (methylation differences < -10, -5 to +5 and >+10 respectively). Of 1539 CGI shores that show increased DNA modification, only 251 genes are differentially expressed (red dots), and of these, 116 genes are upregulated whereas 135 genes are downregulated. b, Summary of the number of canyons in WT LSK cells, including the number of canyons that shrink or expand in Tet2/3 DKO LSK cells compared to WT. c, Average DNA methylation at canyons that decrease in length in Tet2/3 DKO LSK compared to WT LSK cells. The plot illustrates the overall absence of DNA methylation in the canyon center and the increase of DNA methylation at the canyon borders in Tet2/3 DKO LSK compared to control LSK cells. There is a tendency for the gain of methylation in Tet2/3 DKO LSK cells to be more pronounced at the right side of figure, which corresponds to the canyon border towards or within the downstream promoter region of the nearest gene. d, The figure shows the MA plot of Fig. 5a, with the red dots indicating all genes differentially expressed between WT and Tet2/3 DKO LSK cells, and the green dots the genes associated with canyons that shrink (left panel; n=525) or expand (right panel; n=70) in Tet2/3 DKO LSK cells versus WT LSK cells. Black dots, genes that are both differentially expressed and associated with canyons that shrink or expand. Genes associated with shrinking canyons are biased towards downregulation in Tet2/3 DKO LSK cells compared to WT. e, Examples of RNA-seq (top) and WGBS (bottom) results for two downregulated genes (Car2 and Gcnt2) associated with canyons that shrink in Tet2/3 DKO LSK (red) compared with WT LSK (blue) cells.

Supplementary Fig. 19

a

b WT

DKO

c

DKO

γH2AX γH2AX DAPI γH2AX DAPI

γH2AX

WT γH2AX

9 0 3 6 9

Bone marrow

Time (h) 0 3 6

WT

0h

0h

1h

1h

3h

3h

14 h

14 h

22 h

22 h

DKO

γH2AX γH2AX DAPI γH2AX DAPI

γH2AX Actin

Spleen

γH2AX Actin 1 week after injection

GMP cells (ERT2-Cre)

LSK cells (ERT2-Cre)

d

WT

mRNA levels (relative to Gapdh) 18"

16"

14"

5"

***

4" 6"

WT DKO

7" 8"

53bp1

12"

3"

0h

N.D.

8"

N.D.

10"

2"

***

1"

Tet3

6"

4"

0 2 4 6 8 10 12 14 16 18

Tet2

2"

γH2AX γH2AX DAPI γH2AX DAPI

e

0"

γH2AX

DKO

9" 10" 11"

Rad51

12"

1h

13" 14"

Rad54

15" 17"

**

16"

Xrcc2

HR

18"

3h

19"

* 20"

Xrcc3

21" 22" 23"

Rpa1

24"

14 h

25"

* 26"

Xrcc6

27" 28"

NHEJ

29"

Xrcc5

30"

22 h

31"

* 32"

Prkdc Mac-1+ cells (ERT2-Cre)

Supplementary Figure 19. Loss of Tet2 and Tet3 results in accumulation of DNA damage and impaired DNA repair. (a) Combined loss of Tet2 and Tet3 leads to accumulation of γH2AX. Control and Tet2/3 DKO mice were irradiated (6 Gy) at 1 week after pIpC injection and bone marrow (top panel) or spleen (bottom panel) were harvested at the indicated time points. Whole cell lysates were prepared and analyzed for the expression of γH2AX. Actin serves as a loading control. (b) Efficient DNA repair in DKO LSK cells. LSK cells were isolated from control or DKO mice (Tet2-/- Tet3fl/fl ERT2Cre+) at 3 weeks after pIpC or tamoxifen injection, respectively, and DNA repair kinetics in response to 6 Gy of ionizing radiation were assessed by immunocytochemistry. (c,d) DNA damage repair is impaired in myeloid lineage cells upon loss of Tet2 and Tet3. GMP (c) or Mac-1+ cell (d) were sorted from the bone marrow of control and Tet2-/- Tet3fl/fl ERT2-Cre+ DKO mice at 3 weeks after tamoxifen injection and DNA repair kinetics in response to 6 Gy of ionizing radiation were assessed by immunocytochemistry. (e) TET proteins control the expression of DNA repair genes in myeloid cells. Mac-1+ cells were sorted from the bone marrow of WT (Tet2+/+ Tet3fl/fl) and DKO (Tet2-/- Tet3fl/fl Mx1-Cre+) mice at 3 ~ 4 weeks after pIpC injection, and quantitative RT-PCR (PCR with reverse transcription) was performed to assess the expression of genes implicated in homologous recombination (HR) and non-homologous end-joining (NHEJ). Results are expressed as fold change compared with WT cells (arbitrarily set to 1). Data from three independent experiments are shown (Means and SEM). N.D., not detected. *P < 0.05, **P < 0.005, ***P < 0.0005 (Student's t test).

Supplementary Fig. 20

Supplementary Figure 20. Chromosomal aberrations in bone marrow cells from Tet2/3 DKO mice. Red cell-depleted bone marrow cells were isolated from WT mice and sick Tet2/3-deficient DKO mice and subjected to G-banded karyotyping. In one of four bone marrow samples, 6/20 DKO cells examined displayed a structural abnormality of chromosome 3 – an unbalanced translocation of distal chromosome 6 to distal chromosome 3, resulting in an extra copy of the translocated sequences of chromosome 6 and a loss of copy of chromosome 3 distal to the breakpoint on 3.

Supplementary Fig. 21 Original blots for the main Fig. 6a,b,c, h and Supplementary Fig. 19a Spleen DKO

WT

1 2 3 4

MW (kDa)

Weeks:

* n.s. γH2AX

20 15

Actin MW (kDa)

Pre

1 2 3 4

Pre

Weeks:

Pre

Bone marrow DKO WT

1 2 3 4

Pre

Fig. 6a

1 2 3 4

MW (kDa)

* n.s. γH2AX

20 15

Actin

MW (kDa) 50 37

50 37

50 37

* n.s. Actin

37

* n.s.

20

20

γH2AX

15

Long exposure * n.s.

50

Actin

37

* n.s.

20

γH2AX

15

Short exposure

50

Tet2/3 DKO *

n.s. Actin

*

n.s. γH2AX

15

MW (kDa)

MW (kDa)

WT Tet2 KO Tet3 KO

MW (kDa)

WT Tet2 KO Tet3 KO

Spleen Tet2/3 DKO

WT Tet2 KO Tet3 KO

Tet2/3 DKO

WT Tet2 KO Tet3 KO

MW (kDa)

Bone marrow

Tet2/3 DKO

Fig. 6b

Long exposure *

50

n.s. Actin

37

*

20

n.s. γH2AX

15

Short exposure

Fig. 6c Bone marrow DKO

WT Time (h): 0

3

6

Spleen

9

0

3

6

9

Time (h): 0

MW (kDa)

6

9

0

3

6

9

* n.s. γH2AX

20

γH2AX

15

3

MW (kDa)

* n.s.

20

DKO

WT

15

MW (kDa) MW (kDa) 50

50

Actin

37

Actin

37

Suppl. Fig. 19a Bone marrow

20 15

DKO

WT Time (h): 0 3

WT DKO

WT DKO

MW (kDa)

WT DKO

Fig. 6h

6

9

0 3

6

9

MW (kDa) 20

* n.s. γH2AX

n.s.

*

15

γH2AX

MW (kDa) 50 37

Actin MW (kDa)

* n.s. * n.s. Actin

50 37

Spleen DKO

WT Time (h): 0 3 MW (kDa) 20

6

9

0 3

6

9

* n.s. γH2AX

15

MW (kDa) 50 37

Actin

Supplementary Tables Supplementary Table 1. Long-term monitoring of health status of WT, Tet2-deficient and Tet3-deficient mice. WT 1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21

Genotype Tet3fl/fl Tet3fl/fl Tet3fl/fl Tet3fl/fl Tet3fl/fl Tet3fl/fl Tet3fl/fl Tet3fl/fl Tet3fl/fl Tet2fl/fl Tet3fl/+ Tet3fl/+ Tet3fl/fl Tet3fl/fl Tet3fl/fl Tet3fl/fl Tet3fl/fl Tet3fl/fl Tet3fl/fl Tet3fl/fl Tet3fl/fl

Days post injection (DPI) 15 months 15 months 15 months 15 months 15 months 14.5 months 14.5 months 14.5 months 12.8 months 12.8 months 12.8 months 12.8 months 12.8 months 10.7 months 10.7 months 10.7 months 10.7 months 8.4 months 7.3 months 7.3 months 7.3 months

Health status healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy

T2KO 1 2 3 4 5 6 7 8 9 10 11 12

Genotype Tet2-/- Tet3fl/fl Tet2-/- Tet3fl/fl Tet2-/- Mx1-Cre Tet2-/- Tet3fl/fl Tet2-/- Tet3fl/fl Tet2-/- Mx1-Cre Tet2-/- Mx1-Cre Tet2-/- Tet3fl/fl Tet2-/- Tet3fl/fl Tet2-/- Mx1-Cre Tet2-/- Tet3fl/fl Tet2-/- Tet3fl/fl

Days post injection (DPI) 15 months 12.2 months 13.2 months 10.7 months 10.7 months 10.7 months 10.7 months 10.7 months 8.4 months 8.4 months 7.3 months 7.3 months

Health status healthy Found dead Found dead healthy healthy healthy healthy healthy healthy healthy healthy healthy

T3KO 1 2 3 4 5 6 7 8 9 10 11 12 13 14

Genotype Days post injection (DPI) Tet3fl/fl Mx1-Cre 15 months Tet3fl/fl Mx1-Cre 15 months Tet3fl/fl Mx1-Cre 15 months Tet3fl/fl Mx1-Cre 15 months Tet3fl/fl Mx1-Cre 14.5 months Tet3fl/fl Mx1-Cre 10.7 months Tet3fl/fl Mx1-Cre 10.7 months Tet3fl/fl Mx1-Cre 10.7 months Tet3fl/fl Mx1-Cre 10.7 months Tet3fl/fl Mx1-Cre 10.7 months Tet3fl/fl Mx1-Cre 10.7 months Tet3fl/fl Mx1-Cre 10.7 months Tet3fl/fl Mx1-Cre 7.3 months Tet3fl/fl Mx1-Cre 7.3 months

Health status healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy healthy

Supplementary Tables Supplementary Table 2. Hematopoietic parameters after cell transfer experiments a. Haematopoietic parameters in recipients of splenocytes (Tet2-/- Tet3fl/fl Mx1-Cre+). Parameter

WT

DKO

P value

Abnormality

1.95±0.33

98.14±27.54

**, 0.0008

Leukocytosis

RBC (10 /µl)

6

6.27±0.64

3.4±0.28

*, 0.0063

Anaemia

Hemoglobin (g/dL)

8.93±0.78

5.6±0.6

*, 0.0119

Anaemia

Hematocrit (%)

32.69±3.09

21.62±2.46

*, 0.0288

Anaemia

450.25±41.67

240.8±34.63

*, 0.005

Thrombocytopenia

1.16±0.36

6.372±1.07

**, 0.0002

Lymphocytosis

0.67±0.08

79.9±22.96

**, 0.0009

Neutrophilia

0.1±0.012

7.89±2.98

*, 0.0492

Monocytosis Basophilia

3

WBC (10 /µl)

3

Platelet (10 /µl) 3

Lymphocyte (10 /µl) 3

Neutrophil (10 /µl) 3

Monocyte (10 /µl) 3

0.003±0.0016

0.54±0.23

*, 0.0112

7

5.15±0.54

2.59±0.43

*, 0.0059

7

9.92±1.27

31.56±0.35

***,