Title �}_5�R9w]"
要求简练,精确 n#@�Qd!uzM
Compassionate use of bevacizumab (Avastin) in children and young adults with Xt
+9�z�
refractory or recurrent solid tumors. c3r`�T{�Kf
Bevacizumab-induced transient remodeling of the vasculature in neuroblastoma ck�\W'Y*Q7
xenografts results in improved delivery and efficacy of systemically administered nv\K!wZI=b
chemotherapy. �S���a
kew
Proteomics Approaches to the Systems Biology of Cardiovascular Diseases :Qh�rh
(i�
Pre- and post-natal treatment of hemophagocytic lymphohistiocytosis. O8��SE)�R~
Lack of early bevacizumab-related skeletal radiographic changes in children with vrcI�w�C�a
neuroblastoma. pdvnp��zj�
Interleukin-4 activates androgen receptor through CBP/p300 eTuKu(0
E�
Trisomy 8 in an allogeneic stem cell transplant recipient representative of a
�I� Z���w
donor-derived constitutional abnormality. %"eR0Lj+zq
Disruption of diacylglycerol metabolism impairs the induction of T cell anergy L#�z�D�4L�
T cell anergy is reversed by active Ras and is regulated by diacylglycerol kinase- }��pIn3B)�
High-dose conformal RT improves tumor control in patients with prostate cancer aYDo0?k�F'
Vitamin D concentration does not affect the risk of prostate cancer 3bYj�W=_hA
Liver resection with salvage transplantation for hepatocellular carcinoma Ka_;~LS>(�
The impact of histopathologic diagnosis on the proper management of testis neoplasms ��*UJ��4\�
Prostate stem cell antigen is associated with diffuse-type gastric cancer ]!&�$�&t8.
Multiple myeloma: high-risk immunophenotypes identified b?c/�J�{me
Increased c-kit expression predicts poor outcome in acute myeloid leukemia �ixS�r�*+�
Global Analysis of the Meiotic Crossover Landscape �~�$J(it-a
Serum Response Factor Is Required for Sprouting Angiogenesis and Vascular Integrity �*tgu@9��b
Integrin Trafficking Regulated by Rab21 Is Necessary for Cytokinesis +�`_0tM�1
Reduced Translocation of Nascent Prion Protein During ER Stress Contributes to 6��dV )pJd
Neurodegeneration J=t}�9.H~=
Effects of oral niacin on endothelial dysfunction in patients with coronary artery disease: �+{RTz)e?*
Results of the randomized, double-blind, placebo-controlled INEF study. ��� ]%FAJ\
Global experiences with vardenafil in men with erectile dysfunction and underlying ?_i�>�Kx��
conditions. 1��P*hC��<
2 ,(pp+hN��q
Noninvasive cardiac imaging: implications for risk assessment in adolescents and young 6#!CBY�^�{
adults. �%l��!?d`?
Transforming growth factor beta1 T29C gene polymorphism and hypertension: q]I� aRh�o
Relationship with cardiovascular and renal damage. >%om[��]0E
A comparison of hormone therapies on the urinary excretion of prostacyclin and ��D
2kmBZ3
thromboxane A2. Z�|%�h-��~
Repair of an infected aortic aneurysm using an aortic allograft and a venous autograft: �YL��GE{bS
Report of a case. �;=jF9mV�.
Circulating Leptin and Stress-induced Cardiovascular Activity in Humans. oDMPYk�pTu
Effects of aspirin dose on ischaemic events and bleeding after percutaneous coronary BZ�1wE1�t�
intervention: insights from the PCI-CURE study. d#a�/J.Z$A
Long-term cardiovascular outcomes following ischemic heart disease in patients with and >&KH!:�OX|
without peripheral vascular disease. j2<+�[�h-�
Reduced renal function and sleep-disordered breathing in community-dwelling elderly �j�DpA>{O[
men. $Dj8� a\L�
Intracoronary pharmacotherapy in the management of coronary microvascular ��kpIn�_Ea
dysfunction. ����jez0 A
Inhibition of platelet aggregation by combined therapy with aspirin and cilostazol after �mn?F;=�qE
off-pump coronary artery bypass surgery. 1�>j,v��+�
Inhibition of CCR2 Ameliorates Insulin Resistance and Hepatic Steatosis in db/db Mice !�6%?VJB|b
Abstract 要求简洁,连贯 6�/mz.,�g2
The acquisition of metastatic ability by tumor cells is considered a late event in the �fq6Obh=A#
evolution of malignant tumors. We report that untransformed mouse mammary cells that ~3?-l�/��$
have been engineered to express the inducible oncogenic transgenes MYC and KrasD12, or EG�UlLqP6e
polyoma middle T, and introduced into the systemic circulation of a mouse can bypass ,%�*UF6B
M
transformation at the primary site and develop into metastatic pulmonary lesions upon ]��E��X6Y�
immediate or delayed oncogene induction. Therefore, previously untransformed Vb`Vp(�>AU
mammary cells may establish residence in the lung once they have entered the |��6�JKB'�
bloodstream and may assume malignant growth upon oncogene activation. Mammary )�b��Ofs*S
cells lacking oncogenic transgenes displayed a similar capacity for long-term residence in �m6�g�e�
%
the lungs but did not form ectopic tumors. @F<��{/�|P
Almost two decades after CFTR was identified as the gene responsible for cystic fibrosis >0{}tRm-P&
(CF), we still lack answers to many questions about the pathogenesis of the disease, and it "kyCY9)��%
remains incurable. Mice with a disrupted CFTR gene have greatly facilitated CF studies, KU�UA
>�'=
but the mutant mice do not develop the characteristic manifestations of human CF, hT�X�[W%�K
including abnormalities of the pancreas, lung, intestine, liver, and other organs. Because '6dVe��2V�
pigs share many anatomical and physiological features with humans, we generated pigs _Hv+2E[�4Z
with a targeted disruption of both CFTR alleles. Newborn pigs lacking CFTR exhibited w��c;n=�
%
defective chloride transport and developed meconium ileus, exocrine pancreatic u�;_h�%z5K
destruction, and focal biliary cirrhosis, replicating abnormalities seen in newborn humans u[b �|QR=5
3 ���n^4R]9U
with CF. The pig model may provide opportunities to address persistent questions about $�Z�BYO�A�
CF pathogenesis and accelerate discovery of strategies for prevention and treatment. O���:wG/et
Variable lymphocyte receptors (VLRs) rather than antibodies play the primary role in q*&R&K;�q�
recognition of antigens in the adaptive immune system of jawless vertebrates. %lHH�TZ{+�
Combinatorial assembly of leucine-rich repeat (LRR) gene segments achieves the xQu|D>kv87
required repertoire for antigen recognition. We have determined a crystal structure for a �.H�
S6DOQ
VLR-antigen complex, VLR RBC36 in complex with the H-antigen trisaccharide from 1�|MR�
XK�
human blood type O erythrocytes, at 1.67 angstrom resolution. RBC36 binds the 8F}�drK9>F
H-trisaccharide on the concave surface of the LRR modules of the solenoid structure q�� �Q\j��
where three key hydrophilic residues, multiple van der Waals interactions, and the highly �Q1,sjLO-a
variable insert of the carboxyl-terminal LRR module determine antigen recognition and I%��3[aBz4
specificity. The concave surface assembled from the most highly variable regions of the ljKIxSvCFp
LRRs, along with diversity in the sequence and length of the highly variable insert, can Tlw'05\{J�
account for the recognition of diverse antigens by VLRs. Al�-`�}g+^
A 51-year-old man with a diagnosis of myelodysplasia and non-Hodgkin's lymphoma 3�v8LzS�3@
underwent an unmatched allogenic bone marrow transplantation and was treated U] �LD�i�8
posttransplant with chronic immunosuppressive medication. Eight months following �yH�/A9L,Z
transplantation, he presented with progressive dysarthria, cognitive and visual decline. }UhYwJf89�
Evaluation included brain magnetic resonance (MR) imaging demonstrating multifocal vF�27+/2+R
areas of increased T2 and FLAIR (fluid attenuated inversion recovery) signals involving =>�$)F 4LW
the left frontal, parietal, and occipital lobes. The MR lesions demonstrated diffuse z�a_��b jE
increased signal on DWI (diffusion-weighted images) and normal to low signal on ADC nuc����e(R
(apparent diffusion coefficients). Contrast-enhanced T1 images were unremarkable. ^m qE�Ky<�
Lumbar puncture revealed a mild elevation in cerebrospinal fluid (CSF) protein. CSF ���f<YY�o�
PCR assay for viral DNA fragments were negative on two occasions. Serum serology for O��EW'bT)
HIV was negative as well. A brain biopsy was subsequently performed. The clinical and ;k��<dp�7^
neuroimaging differential diagnoses as well as neuropathologic correlation are presented. �Ir9Gg���B
In vitro-generated mesenchymal stem cells (MSCs) initially attracted interest for their y)�G-�6sZ/
ability to undergo differentiation toward cells of different lineages. >P/36���'�
These results suggested that b,�xZY1 a
However, there are still obstacles in p�`"k�=tZ{
The major challenge for successful drug development is identifying delivery strategies @5>#<LV=E#
that can be translated to the clinic. :��
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This review will discuss progress in developing and testing small RNAi-based drugs and A8)�4�nOXM
potential obstacles. Yuv�i{ ��0
This review highlights what *1)>He�$qL
In addition, there are indications that ]~�T�smR[�
Proper consideration of all of these issues will be necessary in #Bd]M#J17a
These studies provide
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This paper presents the potential applications and the hurdles facing anti-HCV siRNA I�3�t5S;_8
drugs. �-k�'<6�op
The present review provides insight into the feasible therapeutic strategies of siRNA N^L�@MR�
-
technology, and its potential for silencing genes associated with HCV disease. ��x?��h/e;
4 <Ky-3:pxeM
A basic problem in the design of xx is presented by the choice of a xx rate for the ��.U1wVI�M
measurement of experimental variables. �z��x.�qN
This paper examines a new measure of xx in xx based on fuzzy mathematics which Itl�8#LpLM
overcomes the difficulties found in other xx measures. �|2�(�q�9j
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The method involves the construction of xx from fuzzy relations. ZEqW*piI��
The procedure is useful in analyzing how groups reach a decision. *;<fh,wO�k
The technique used is to employ a newly developed and versatile xx algorithms. (5y�M%H8�:
The usefulness of xx is also considered. �}`tS�RB7
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The analysis is useful in xx and xx problem. ;4�F6
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A model is developed for a xx analysis using fuzzy matrices. QS#@xh�H��
Algorithms to combine these estimates and produce a xx are presented and justified. u�?^�V4 +V
The use of the method is discussed and an example is given. �iN;Pg�_Kq
Results of an experimental applications of this xx analysis procedure are given to �S=@�+�qcI
illustrate the proposed technique. h@���,�ja�
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achieving a hierarchical system of objectives are evaluated. RX���gb/VR
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requiring mechanical ventilation, which greatly increases mortality >�"�W^|2�R
The cause of respiratory failure in patients with AKI is incompletely understood �LU3�p�CM{
However, lung injury also occurs after ischemia–reperfusion injury of other organs such &PM��Q�]B�
as the liver, gut, and hind limb k+QGvgP[4@
We have demonstrated previously that wE
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Polyphenolic compounds are vasodilators and help to lower the risk of cardiovascular O-,�
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diseases. ! ._�q8q\�
Taken together, our novel findings suggest that the EDR induced by the strawberry #:�6��-�O�
extract was mediated by activation of the PI3 kinase/Akt signaling pathway, resulting in .�s{�"NqRA
phosphorylation of eNOS. p��?gm�=b#
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The ultimate goal of the xx system is to allow the non;experts to utilize the existing a�_��N7��X
knowledge in the area of manual handling of loads, and to provide intelligent, _�H$Lu4b)N
computer;aided instruction for xxx. 6A"$9s��j6
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for the xx. *OLqr/ �yb
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fuzzy data: xx.
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deiodinase activity due to a mutation in SBP-2 �4�!
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xx 6H��|1Ir�G
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cellular and molecular aspects of local control of thyroid hormone signaling provided by }$_@yt<{W@
deiodinases. C ��hF~��
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well in methodological aspects as in concrete applications. >V6�t
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MATERIALS AND METHODS �W�8`6��O2
Materials �tW��l'�)^
Chemicals were purchased from Sigma (St Louis, MO), if not stated otherwise. ir}*�E�=�*
Experiments were conducted in accordance with the NIH Guidelines for the Care and Use �O�E[7fDe'
of Laboratory Animals. `d�F����~'
CsA, EGF, PD98059, U0126, AG1478, Wortmannin, and LY294002 were from �[� {"�x{;
Calbiochem (San Diego, CA, USA). Anti-ERK1/2 and anti-Ras were from Transduction 3W �]zL�Un
Laboratories (Franklin Lakes, NJ, USA). Anti-phospho Raf-1 (Ser259), anti-phospho 6��V�QQ�I9
Raf-1 (Ser338), anti-phospho PKB/Akt (Ser473), anti-PKB, anti-phospho EGFR (Tyr1068), N
(\n$bpTt
anti-phospho ERK1/2 (Thr202/Tyr204), anti-PI3K 110 , anti-p53, and anti-phospho C�<C^�7-5�
MEK1/2 (Ser217/221) were from Cell Signalling (Danvers, MA, USA). Anti-MEK and c�{`!$Z'k<
anti-Raf-1 (C12) were from Santa Cruz (Santa cruz, CA, USA). Apigenin and all other C�&@'o�Lr�
reagents were from Sigma (Saint Louis, MO, USA). GYy�8kp84�
Animal ?�.Ob�HV*k
Eight- to ten-week-old male C57BL/6 mice (wild-type) and IL-6-deficient mice T/u61}'U�{
backcrossed over eight generations on a C57BL/6 background were used x���| D|d}
Mice were maintained on a standard diet and water was made freely available. �Qd~7OH4Lp
All experiments were conducted with adherence to the NIH Guide for the Care and Use �(�MqQ�3ys
of Laboratory Animals. f@9XSZ<.71
The animal protocol was approved by the Animal Care and Use Committee of the KN@ [hb
7%
University of Colorado rpEI�DhH�v
Three surgical procedures were performed as described previously:5 (1) sham operation, G]x�YQ�]�
(2) ischemic AKI, and (3) bilateral nephrectomy. �/Xc9�}~t6
The abdomen was closed in one layer. v�nf2Z�,f%
Sham surgery consisted of the same procedure except that clamps were not applied. �GGLSmf�b)
9 m�0�W3�pf�
For bilateral nephrectomy, renal pedicles were tied off with suture and then cut distally. �_8SB�+�s*
The ureters were pinched off with forceps and the kidneys removed. H��#X*�O�J
Serum was collected as described previously.5 Blood urea nitrogen and creatinine were ;9#�W�#�/B
measured using an autoanalyzer (Beckman Instruments, Fullerton, CA, USA). p4�\s�KF8-
Serum IL-6 was measured by ELISA according to assay instructions (R&D Systems, �T�X��d6o=
Minneapolis, MN, USA). w|I5x}Z
FG
Five-micrometer sections of paraffin-embedded lung tissue were stained with q|k�ls�up�
hematoxylin and eosin using standard protocols. Neutrophils were counted on the basis of �^v5]A�q~X
morphological criteria; at least 50 high-powered fields ( 40) were counted per slide. n<)A5UB5-�
Frozen lung was prepared for ELISA as described previously.5 Supernatants were /EH�O(d!�<
analyzed for protein content using a Bio-Rad DC protein assay kit (Hercules, CA, USA). t0xE&�#4��
KC and MIP-2 were determined by ELISA (R&D Systems, Minneapolis, MN, USA). 6�o]{< T/'
One-fourth lung was used to determine MPO activity as described previously. eC� 2~&:$L
Frozen lung was homogenized in radioimmunoprecipitation assay buffer with protease
5�U�hxl^c
inhibitor; western blotting was performed as described previously.49 Goat anti-murine V\n!?1{kdF
ICAM-1 polyclonal antibody (R&D Systems, Minneapolis, MN, USA; 1:2000) or rat N*PJ m�6�-
anti-murine VCAM-1 monoclonal antibody (R&D Systems; 1:1000) were used. g@t..x��J,
A total of 20 g anti-IL-6 antibody vs IgG control (eBioscience, San Diego, CA, USA) _h��,X3P��
was administered to wild-type mice by tail vein injection 1 h before surgery, wm��Mn1q0F
intraperitoneally at the time of clamp removal (ischemic AKI) or nephrectomy (bilateral a3:45[SO4e
nephrectomy) and intraperitoneally 1 h following surgery (60 g total). 5�&�A�' +]
Experimental groups #;1RStb:zj
STZ-induced diabetic rats, a model of partial type I diabetes: SD rats received a single
C>-}BeY!
intraperitoneal injection of freshly prepared STZ (65 mg kg-1 body weight, dissolved in W�?N+7�_%'
100 mmol l-1 citric acid, pH 4.5), and confirmed 2 days later by PP blood glucose iY�d�g1���
(>250 mg dl-1). Hit�)mwfYE
CTR rats: Vehicle-injected SD rats after 2 to 7 days, 14 to 30 days, and 90 days served as X�=Y(,ZR(&
CTR for the 2 and 7 days STZ, the 14 and 30 days STZ, and for the 90 days STZ, ��1n*"C!�q
respectively. �=_6 Q��26
Insulin treatment in STZ: Glc was normalized in seven animals during 12–14 days of 64�y9.P�Y�
STZ by subcutaneous insulin implants (2U day-1; Lin Shin Canada, Ontario, Canada). � YO�f�Ya�
Cell Culture t82*rC�IB{
Immortalized cells from the convoluted portion of mouse kidney proximal tubule >$3�� =yw%
PKSV-PCT cells (PCT3 clone) were cultured in a medium A (DMEM/Ham's F12 (1:1, ]|I�e��E!6
v/v), 20 mM HEPES, 2 mM L-glutamine, 12.5 mM D-glucose, 60 nM sodium selenite, �O��zH\�YN
5 g ml-1 transferrin, 50 nM dexamethasone, 100 U ml-1 penicillin, and 100 g ml-1 uzp�\<\d-t
streptomycin), supplemented with 2% fetal bovine serum, 5 g ml-1 insulin, 10 ng ml-1 `USze0"t0:
EGF, and 1 nM triiodothyronine at 37°C in a 95:5 air/CO2 water-saturated atmosphere. �.G<Or`K^i
For all experiments, cells were seeded at 0.2 106 cells/ml and after 24 h with complete :a=]<�_*x�
medium cells were starved for 16 h in medium A supplemented with 0.1% fetal bovine ��>*|�Eyv_
10 ��od�!s5f!
serum but not insulin, EGF, or triiodothyronine. CsA was dissolved in ethanol and all the `$J
�OFLa�
pharmacological inhibitors were in DMSO. In all cases, controls were carried out with q}E'x�/s2m
cells treated with the corresponding vehicle alone. After treatments, cells were washed ds2x��l7jg
twice with cold phosphate-buffered saline (PBS) and harvested with lysis buffer as in �^Y8G��}Z|
Llorens et al Q�d�D��@�[
Cell viability �!_dW
���`
After treatments, PCT3 cells were harvested and washed twice with cold PBS, and the '1G0Y�fG}n
viable cells were counted with Trypan Blue Dye (Gibco-Life Technologies, Grand Island, 5m��Z�9rLn
NY, USA) in a Neubauer chamber. Living cells exclude the dye, whereas dead cells will �N>@.(�f&w
take up the blue dye. For Hoechst staining, cells seeded in six-well dishes were washed Z�]O�X6�G
twice with PBS and fixed for 15 min with 4% paraformaldehyde at room temperature. ��09iD| $~
Then, cells were washed twice again with PBS and stained with Hoescht (5 g ml-1 in 1bCS4fs^�>
PBS) for 5 min. 1@+�&6�U�C
Western blots/ Immunoblot B]>�rcjD��
The protein content of cellular extracts was quantified by the Bradford assay.44 Ax4;��[K\Q
Twenty-five microgram of total cell extract protein was run on SDS-polyacrylamide gel (+�TL
]�9P
electrophoresis gels, transferred onto polyvinylidene difluoride membranes, and `�K�2vG`c�
incubated with the corresponding antibodies. The membranes were developed with the ,`���$��2�
enhanced chemiluminescence method (Pierce, Rockford, IL, USA). q�}&+{dN\1
Supernatants of growing or growth-arrested cells were centrifugated for 5 min at 10 000 g. A.!3�{pAb�
The cells were lysed as described. The proteins from supernatant and cell lysates were ~�}�G#ys\1
concentrated using heparin sepharose. The heparin sepharose was washed four times with c[?&;# feV
phosphate-buffered saline containing protease inhibitors, dissolved in phosphate-buffered �z+?�48��}
saline/protease inhibitor and incubated with 500 g protein over night at 4°C. The �Mi[,-8Sk�
complexes were washed with phosphate-buffered saline/protease inhibitor and the �b�]W�vKdq
proteins were eluated with 100 l Laemmli buffer without bromophenol blue (10 min j�2��#B �l
95°C). A 30 l probe was loaded in each lane and western blot analysis was performed as lF$$��~
G�
described, using a polyclonal antibody against CCN3 (K19M), which recognizes a ;��F�jI�!V
C-terminal 19-aminoacid peptide of human CCN3. As a positive control, a supernatant w6l56�CB�`
from adrenocortical cell cultures, which are known to secrete CCN3, was used. DEen�vS`,P
Cells were lysed in 0.5% (volume/volume) Triton X-100 lysis buffer and immunoblot �;�:Y/�"5h
analysis was done as described43. Immunoprecipitation with anti-CrkL or control rabbit �,\PT�n7�_
antiserum was done as described44. Antibodies to the following were used: j<vU[J+gx~
phosphorylated Erk (910L; Cell Signaling); phosphorylated Jnk (V7932; Promega); Erk �GS!�1K(�7
(13-6200; Zymed); Jnk1 (sc-474), H-Ras (sc-35), C3G (sc-869), CrkL (sc-319), Nb��m$t��a
RasGRP1 (sc-8430) and DGK- (sc-8722; all from Santa Cruz Biotechnologies); and ;BEX|w�x�n
DGK- (a gift from H. Kanoh, Sapporo Medical University, Sapporo, Japan). Images O�lq`mlsK�
were scanned, followed by densitometry analysis with UN-SCAN-IT software (Silk M3q7{�w*bM
Scientific). ,,V���uv�n
11 z�vbz3��a�
Purified splenic T cells were stimulated for various times with 5 g/ml of anti-CD3 &_�Gu'A({J
(500A2; BD Pharmingen) and were lysed in 1% Nonidet P-40 lysis buffer (1% @<p9��O��0
(volume/volume) Nonidet-40, 150 mM NaCl and 50 mM Tris, pH 7.4) with protease J2$�=H1-��
inhibitors. Proteins were resolved by SDS-PAGE and were transferred to a Trans-Blot %VgK�::)�r
Nitrocellulose membrane (Bio-Rad Laboratories); membranes were probed with l�,��E4h-$
antibodies specific to phosphorylated Erk (91015; Cell Signal Technology) and '�]vMOGG
�
phospholipase C- 1 (05-163; Upstate Biotechnology). Membranes were stripped and #r80F�VwiD
were reprobed for analysis of total Erk (SC-16982; Santa Cruz Biotechnology). Activated !%G;
t$U=M
Ras in cell lysates was determined by glutathione S-transferase–Raf—Ras-binding ~�ZRtNL9��
domain precipitation assay as described VD2o#.7*eu
Immunofluorescence microscopy. �wRE2rsXoU
Analysis of protein localization in 2C T cell–P815.B71 cell conjugates was done as 7e<\11uI]a
described29. P815.B71 cells were labeled with CMAC (7-amino-4-chloromethylcoumarin) ~RnBs�`&�!
Cell-Tracker Blue (Molecular Probes) and were mixed with equal numbers of anergic or ���&�d[�%�
in vitro–primed 2C Rag2-/- T cells. After approximately 8 min, cells were fixed, were
q&E�wD(k�
made permeable and were stained with anti-GRP1 and anti-talin (Santa Cruz �L�wE�c*79
Biotechnologies) and with species-specific secondary antibodies conjugated to A,GJ6q�p3
fluorescein isothiocyanate or phycoerythrin, respectively. Samples were analyzed with a P�,��SI0$Z
Zeiss Axiovert 100 microscope, and 15 conjugates were typically assigned scores. C�<iOa)_@Q
Slidebook software (Intelligent Imaging Innovations) was used for image capture and %J|
xPp)��
deconvolution analysis. ImageJ 1.36b software (US National Institutes of Health) was N�`i`�[� f
used for quantification of pixel intensity. �>�R8eAR$N
Measurement of ROS generation ( 0Z3Ksfj1
The assay is based on the incorporation of 2',7'-dichlorofluorescein diacetate into the cell. d9�uT*5�f�
H2O2 and peroxidases are able to oxidize the cleaved DCFH to DCF, which is highly �~6:y@4&�F
fluorescent at 530 nm. To measure CsA-induced ROS generation, cells were washed ^�D�hu8C(�
twice with PBS, and fresh medium containing 20 M 2',7'-dichlorofluorescein diacetate <�\S�
�j�5
was added to previously treated cells. After 30 min cells were washed again, tripsinized, ��t>>\U X�
and resuspended with cold PBS. Fluorescence was measure by flow cytometry on a (L6�*#!Dt�
FACScan flow cytometer. $8�,/�[V
A
Raf-1 activity ='|H�UxF�i
Raf-1 immunoprecipitation and kinase assay were performed as described previously.45 n�`)wD~m�k
Immunoprecipitated Raf was incubated for 30 min at 30°C with 0.8 mM ATP, 10 g ml-1 ��B[Fuy�y?
GST-MEK, and 100 g ml-1 GST-ERK2. An aliquot of the supernatant was used for #NLL�l�E�E
ERK2 activity assays using 0.5 mg ml-1 myelin basic protein and 0.1 mM [ -32P] ATP �y[@<g��oT
(400 c.p.m. pmol-1). After 15 min incubation at 30°C, 12 l of 5 Laemmli loading yS:1F
PA$_
buffer was added to the tubes and the mixture analyzed by SDS-polyacrylamide gel �yD9<-�B<)
electrophoresis. Radiolabeled bands were quantified in a PhosphoImager. b/Z��0{3�8
12 a0��ze7F<(
Semiquantitative RT-PCR. 4?�^t�=7N�
Total RNA was isolated from freshly isolated thymocytes. Then, cDNA was prepared &$�<�/|F)y
with the M-MuLV reverse transcriptase and random primers according to the l6Q75i)�eF
manufacturer's recommendations (New England Biolabs). Semiquantitative PCR analysis �a,N?Gx�K~
of Tcrb VDJC (where 'C' is the constant region) and Cd3e cDNA was done as described51. +t�XOP|��X
[32P]dCTP (GE Healthcare Life Science) was incorporated into PCR products for O/=i'0X�v�
semiquantitative detection by autoradiography. '�
�{:Yg3K
Real-time quantitative RT-PCR �W}5�H'D
�
Total RNA was isolated from HMC or rat mesangial cells using the Invisorb Spin vY�Nh0)$%F
Cell-RNA Mini Kit (Invitek, Berlin, Germany) or from isolated glomeruli using the Vhs:X~�=qL
RNeasy Mini Kit (Qiagen, Hilden, Germany). RNA purity determination, cDNA L){r�v)?="
synthesis, and RT-PCR were performed as described.16 Primer sequences are listed in XHlx�89�v7
Table 2. Glyceraldehyde-3-phosphate dehydrogenase cDNA amplification was used as an �Y(]&j`%��
internal standard. #�)��B�dN�
Total RNA was isolated from the frozen kidneys as described by Chomczynski and a,U �=irBA
Sacchi47 and quantified by a photometer. One microgram of the resulting RNA was used ,SAS\�!hsE
for reverse transcriptase (RT)-PCR. The cDNA was synthesized by MMLV reverse 5)yQrS !{:
transcriptase (Superscript-Invitrogen, Carlsbad, CA, USA). For quantification of renin \8!&X��c�A
mRNA expression (sense: 5'-ATGAAGGGGGTGTCTGTGGGGTC-3', antisense: �?�)cNe:KY
5'-ATGCGGGGAGGGTGGGCACCTG-3'), real-time RT-PCR was performed using a �B9�4m���h
Light Cycler Instrument (Roche Diagnostics Corp., Basel, Suisse) and the QuantiTect /.\$%b�ua�
SYBR Green PCR kit (Qiagen, Hilden, Germany), with GAPDH (sense: M,Px.�@tw.
5'-TTCATTGACCTCAACTACAT-3', antisense: 5'-GAGGGGCCATCCACAGTCTT-3') 1lNg} !)[K
as a control. PCR was run for 30 cycles with 15 s per 95°C denaturation, 20 s/58°C 4>�gMe3]0�
annealing and 20 s/72°C elongation. To verify the accuracy of the amplicon, a melting �9�zkR�)C�
curve analysis was done after amplification.Total renin mRNA content per kidney was �BV&}�(9z�
calculated from the yield of RNA extracted from the whole kidneys times the renin �h<9���h
2
mRNA estimate obtained from the defined amount of RNA used for RT-PCR real time OX�?9 3AlG
measurement. For the RT-PCR real-time measurements, a pool of RNA from adult mouse Z<|ca�T]Q(
kidneys was generated, which served as standard for all RT-PCR runs. Thus, all renin NDRk%_Eu�(
mRNA levels for the developing kidneys were estimated relative to the levels in adult 'Z�7oP�q�6
kidneys. 'P�lKCn`(w
In vitro anergy assay. `\&q�k)�ZP
Wild-type, Dgka-/- and Dgkz-/- splenocytes were stained with 5 M CFSE, were w>X33Ff]8@
stimulated for 72 h with anti-CD3 (1 g/ml; 2C11) along with CTLA-4–Fc (5 g/ml), s�&lZxnIjc
were stained with allophycocyanin-conjugated anti-CD4 and were analyzed by flow �T���"Wq:�
cytometry. Cell division was assessed by CFSE dilution after gating on live CD4+ cells. ;1cX|N��=�
Alternatively, cells were stimulated for 72 h and were pulsed with 1 Ci/well of f��j 19U9R
[3H]thymidine for the final 8 h of stimulation, and proliferation was assessed by tritium .l*�]W!L]�
incorporation with a scintillation counter. For restimulation analyses, cells were e�@�L'H)w,
13 y-"*[��5{W
prestimulated with anti-CD3 plus CTLA-4–Fc, then after 72 h, CD4+ cells were purified u9>.x
zY�G
by negative selection (with fluorescein isothiocyanate–conjugated anti-CD8, anti-B220 ''wW�w(2�O
(RA3-6B2; BD Pharmingen), anti-DX5 and anti-CD11b (M1/70; BD Pharmingen), ;2}0�H�r'|
followed by depletion with anti–fluorescein isothiocyanate magnetic beads) and were �g����B�<p
allowed to 'rest' overnight at 37 °C. Live cells were then counted by Trypan blue )j�@k[}R#g
exclusion, and equivalent numbers of live cells were dropped onto monolayers of bone o)?"P;UhJX
marrow–derived macrophages coated with anti-CD3 (1 g/ml) and anti-CD28 (0.5 bs]ret$?(q
g/ml). After 24 h, supernatants were collected and IL-2 was quantified by ELISA ^?to�TU� �
according to the manufacturer's protocol (R&D Systems). �&tQ,�2R�T
Three-dimensional reconstruction OR( �)D~:n
Serial sections of kidney specimens were fixed and stained for renin and for SMA as �r[M�]2�h�
described above. Digitalization of the serial slices was performed using an AxioCam T�RAs5I�%�
MRm camera (Zeiss, Jena, Germany) mounted on an Axiovert200M microscope (Zeiss) t_,i�V9NrZ
with fluorescence filters for renin and SMA (TRITC: filter set 43: Cy2: filter set 38 HE; ,US~p_�M�!
Zeiss). After acquisition, a stack of equal-sized images was built using the graphic tool ��*=S\jek�
ImageJ (Wayne Rasband, NIH, Bethesda, MD, USA). The equalized data were then 4lb3quY$Us
imported into the Amira 4.1 visualization software (Mercury Computer Systems Inc., T[<ll��h'+
Chelmsford, MA, USA) on a Dell Precision 690 computer system (Dell, Frankfurt, r�em&F'x0V
Germany), and subsequently split into the renin and SMA channels. After this step, the 8�+
B.��x�
renin and SMA channels were aligned. In the segmentation step, the SMA and renin UY{
Uo@k9x
data sets served as a scaffold and were spanned manually or automatically using F�m,A<+l@u
grayscale values. Matrixes, volume surfaces, and statistics were generated from these �J}`K&DtM9
segments. =t�&B8�+6�
Restimulation assay after in vivo immunization. zG@9-�s* L
For analysis of T cell priming in vivo, CD4+ T cells were collected from naive, primed or ,��Xk8{�=�
tolerized recipient mice on day 15 after immunization. Proliferative responses were d)�r=W@tF]
measured by culture for 72 h of CD4+ T cells (3 106 cells/ml) with irradiated (3,000 rads) ����
)��Ah
APCs (10 106 cells/ml) and OVA(323–339). The number of KJ1-26+ cells for each .XUR�I#��b
group of recipient mice was determined by flow cytometry and proliferation was 1(hgSf1�WH
normalized to the number of input KJ1-26+ cells. Supernatants were collected from plates tI{
n�!
and cytokine concentrations were measured by ELISA. WU#bA�|Cf�
Flow cytometry. cK�F02?)TX
For analysis of surface antigen expression, mAb to CD4 (JK1.5; eBioscience) and mAb Wz:M�Pdz3(
KJ1-26 (KJ-126; Caltag) were used. For intracellular IL-2 staining, T cells were -h�p�,O?PM
restimulated for 24 h in vitro with OVA(323–339) in the presence of APCs as described f��BD�5K�3
above. Brefeldin A (eBioscience) was added for the last 6 h of the culture. Cells were 8����DLR�
collected and were stained with allophycocyanin-conjugated mAb to CD4 and fluorescein �cdzzS�?$)
isothiocyanate–conjugated mAb KJ1-26. Then, cells were fixed, were made permeable ��+*)B;)�P
and were stained with antibody to IL-2 (clone JES6-5H4; eBioscience) according to the #�dW$"u���
manufacturer's instructions. �:;{U2q+��
14 4^70�r9hV9
TH1 cells transduced with adenovirus vector encoding GFP were analyzed with a XuR!9x�^�5
FACScan (BD Biosciences). A total of 1 104 events were acquired, and data were 7�9:x>�i=�
analyzed with CellQuest software (BD Biosciences). MV9{�>xX��
Splenic and lymph node samples depleted of thymocytes and red blood cells were stained r�^�#.�yUz
with fluorescence-conjugated anti-CD3 (2C11), anti-CD4 (GK15), anti-CD8 (53-6.7), Xd|@w{.�m*
anti-CD25 (7D4) and anti-CD44 (552407; all from BD Pharmingen). A three-color ;1��3�lu�1
FACScan (Becton Dickinson) was used for flow cytometry, and data were analyzed with 0~Yg={IKhK
FlowJo 4.6 (TreeStar). c��QgmRHZ]
A FACSCalibur (Becton Dickinson) was used for flow cytometry. Human cells from jh\q2E~�,`
transplanted NOD-SCID mice were assessed with phycoerythrin–cyanin 5–conjugated �}A��x$}#�
anti–human CD45 and phycoerythrin-conjugated anti-CD19, anti-CD33, anti-CD36 and =,gss&J!!�
anti–glycophorin A (Becton Dickinson). EGFP fluorescence was detected with channel K.l?R#G`,F
FL1 calibrated to the fluorescein isothiocyanate emission profile. During quadrant rCYNdfdp�p
analysis, only fluorescence excluding more than 99% of isotypic control events was �j]Rl1~+M�
considered specific. Cell Quest Pro software (Becton Dickinson) and FlowJo (Tree Star) /,E%�)�K�;
were used for data acquisition and analysis. QnaMj
Dh$6
Mammalian expression plasmids and transfection. ��������fB
For generation of the plasmid expressing Smad3 shRNA, the following specific �"�~d)�$]+
oligonucleotides were used: upper, .o|�Gk
�5)
5'-GATCCACCTGAGTGAAGATGGAGATTCAAGAGATCTCCATCTTCACTCAGG �
Q�9%N>h9
TTTTTTTACGCGTG-3'; lower, hb�E;zY%hP
3'-AATTCACGCGTAAAAAAACCTGAGTGAAGATGGAGATCTCTTGAATCTCCA ;\�Wg>�s�q
TCTTCACTCAGGTG-5'. These were cloned under control of the U6 promoter into the TK�Ru^KH9�
pSIREN-DNR-DsRed expression vector (Clontech, BD). Vector expressing shRNA <ezvz�..�g
specific for luciferase served as a control. Smad3-Tm was subcloned into the X��5>p~;[9
pIRES2-EGFP vector (Clontech, BD); empty vector served as a control. Purified �YroKC+4"i
DO11.10 or DO11.10p27 T cells were transfected with plasmids by nucleofection with z%*ZmF�^K�
the Amaxa nucleofection apparatus, according to the manufacturer's instructions (Mouse �c?<FMb3�]
T Cell Nucleofector Kit Amaxa Biosytems). Purified T cells were suspended in N<N�!�i�t�
nucleofector solution (3 106 cells/100 l) and were mixed with 3 g of plasmid. *e
_ /D$SC
Samples were transferred into cuvettes, were transfected with nucleofector program X-01 V-7�!�)�&q
and were then immediately transferred into 12-well plates and were cultured in J]N�-^ld\\
nucleofector medium for 3 h. Then, cells were collected and counted and were d�x
���Mz!
immediately transferred into syngeneic recipient mice (3 106 cells per mouse). At 3 h �F�o;�xA��
after adoptive transfer, mice were given priming or tolerizing treatment in vivo according DOU\X �N��
to the standard protocol described above. Lymphocytes were isolated from draining DJrA�@hm/Y
lymph nodes at day 5 of the treatment, CD4+ T cells were purified and transfection evi�m�n��V
efficiency was assessed by flow cytometry. The range of transfection efficiency was #[I�`V�A\x
69–75% (Supplementary Fig. 4 online). Smad3-knockdown and control-knockdown �mI"�|^!L
DO11.10 cells and DO11.10 cells transfected with Smad3-Tm and vector control were p(U'�c}@2�
selected by cell sorting. The resulting CD4+ T cells (2 106 cells/ml) were restimulated �HK:?Y[ebs
with OVA(323–339) (5 g/ml) in the presence of irradiated APCs in vitro. GbStq�R~^#
15 �<5C3c&sds
Luciferase assays. Nz5gu.a6{L
CAR IL-2–Luc TH1 clones were transduced with vectors, were stimulated for 20 h and XL} oYL]}&
were resuspended in serum-free DMEM in luminometer cuvettes (BD Biosciences). An p�1G!-��\l
equal volume of Bright-Glo luciferase assay reagent (Promega) was added to each sample, 1�{nXmtvr�
followed by thorough mixing. After 2 min, samples were analyzed with a monolight 2010 �-- �
_,;
Luminometer (BD Biosciences). O��v?k4�kJ
Analysis of cell divisions in vivo. M@s2T|bQ�w
Purified T cells from DO11.10 and DO11.10p27 mice (10 106 cells/ml) were labeled ��L6 h�Tz'
for 30 min at 37 °C with the intracellular fluorescent dye CFSE (5 M 5(and �� �b.C!4^
6)-carboxyfluorescein succunimidyl ester; Molecular Probes). Then, cells were washed Bv!j.$0�d{
twice with cold RPMI 1640 medium containing 10% FCS, were resuspended in PBS and ;wT�l#\|w0
were transferred intravenously into BALB/c mice (5 106 cells per mouse). Syngeneic $]xe,}*�Af
hosts were left untreated (naive) or were treated with PBS followed by immunization 1(rH5�z�'F
with OVA(323–339) (primed) or with CTLA-4–Ig plus mAb to CD40L followed by �`�){*�JPl
immunization with OVA(323–339) as described above (tolerized). Then, 3 d later, 9
<�\�wa/#
lymphocytes were isolated from the draining lymph nodes of the BALB/c hosts. The AP/5,�M<��
number of cell divisions on CFSE-stained cells and the percentage of cells that had }2V��|B��4
undergone a specific number of divisions were determined as described43. Cells were also >RF�[0s�'-
stained with mAb KJ1-26 and CFSE analysis of KJ1-26+ T cells was done by flow H.w�p{�m{�
cytometry. (��j��}�"1
Adenovirus vectors. �*��4]�I#N
The cDNA encoding Ras61L was provided by F. Fitch (University of Chicago, Chicago, ��VJZ�� �
Illinois). The dominant negative Cbl construct was generated by RT-PCR with cDNA -4;{QB���?
from TH1 clones as a template and the following primers (upper case, restriction enzyme _YO��`�x�
sequences; underlining, Myc tag sequence): S-'iOJ�1]�
5'-GGGGTACCatggagcagaaactcatctctgaagaggatctggccggcaacgtgaagaaga-3' (forward) and 3
D;\�V&([
5'-ATAGTTTAGCGGCCGCtcaatcttgaggagttggtt cacataa-3' (reverse). The cDNA F~{yqY5�]n
encoding DGK- was a gift from M. Topham (University of Utah, Salt Lake City, Utah) C!�RxMccTh
and was used as a template to introduce an N-terminal Myc epitope tag by PCR. The (#LV*&K%IC
sequences of all PCR products were confirmed before subcloning. Construction of �9(AN�h�G�
recombinant adenovirus vectors was done with a two-cosmid system that has been fL�c�t!H3�
described42. �^<[o�Ki;>
Adenoviral transduction of CAR T cells. p2�4s�W�Df
TH1 clones were purified from passage cultures by Ficoll-Hypaque centrifugation. >Y)jt*vQ��
Primary CAR 2C Rag2-/- CD8+ T cells were isolated from splenocytes by negative ��|UB�R�8�
selection with magnetic beads and antibody 'cocktails' (Stem Cell Technologies). CAR Q5{i#F7nJm
TH1 cells were transduced with adenovirus vectors at high cell density (1 107 cells/ml) �~U ?cL-`n
in DMEM containing 2% (volume/volume) FCS and were incubated for 1 h at 37 °C, �m:II��<tv
16 J�U/K\S2%,
followed by an overnight 'rest' at 37 °C in DMEM containing 5% (volume/volume) FCS �B5zu�?�AG
at low cell density (4 105 cells/ml). {C|��#<}1�
Lentivirus production and infection protocols. L�?4�c8�!Q
A third-generation lentiviral vector encoding EGFP expressed from the human s1:�UCv-�%
phosphoglycerate kinase promoter was used as described29, 33. Cell populations were W&T��Pr
B�
incubated overnight (about 16 h) in X-VIVO-10 medium (BioWhittaker) supplemented o^d(mJZ.F~
with 1% BSA (Stem Cell Technologies) and L-glutamine (Invitrogen) with viral V��,*�YM��
supernatant (multiplicity of infection of 130–180). Viral concentrations of 1.0 108 to 1.8 kO~x�E�-(=
108 viral particles/ml, 2.0 107 to 4.4 107 viral particles/ml and 0.9 108 to 1.6 108 W4�46�;)?5
viral particles/ml and cell concentrations of 0.7 106 to 1.1 106 cells/ml, 1.0 105 to 2.5 T_y '�cv�h
105 cells/ml and 0.7 106 to 1.4 106 cells/ml for CD34+CD38lo, CD34+CD38- and Lin- =J�X.*
MEB
cord blood, respectively, were maintained. The efficiency of gene transfer was estimated o�/2\8�� �
by progenitor cell assay as described33. ��J$j�&j`�
Apoptosis induction. c�^R�z�?2x
Spontaneous apoptosis of PMNs was detected after 22 h of incubation in culture media. $9M>�B<�]�
In some experiments, zVAD-fmk (10-50 M), TNF (40 ng/ml), resolvin E1–methyl ester, 4U�S8B�=jk
aspirin-triggered lipoxin A4 analog, PD1–methyl ester (10 nM) or TGF- (10 ng/ml) was V�.:��a6>]
added. Vehicle treatment was 0.05% (volume/volume) ethanol. Peripheral blood T cells >.\G/'�\?�
were activated by incubation for 3 d in 24-well plates coated with anti-CD3 (5 g/ml; �#xm<|s ��
R&D Systems). Jurkat cells or activated peripheral blood T cells were incubated for 4–48 _ZC4O&�fL�
h with staurosporine (1–2 M) or Fas ligand (0.05–5 ng/ml), after which cells were ��mQ�('X~l
collected and used for flow cytometry or binding assays. In some experiments, eLL>�ThMyW
zVAD-fmk (10–50 M; R&D Systems) was added to cells 20 min before the addition of J &u&G7#S
apoptosis-indu �h���c`9�Y
Mice strains and genotyping. WK�:~�2m&y
The 129/Sv Rhoh-/- mice were generated by Targeting Laboratory. The entire coding 2:&8�F�d�U
region of mouse Rhoh is in its third exon; the targeting vector was designed to replace the lk���1c�2�
third exon of Rhoh with a neomycin-resistance cassette. The genotypes of Rhoh PF1!aAvVb�
gene-targeted embryonic stem cells and transgenic mice were determined by Southern `a�3q)}*Y�
blot analysis of DNA digested with SpeI using a 5' Rhoh genomic DNA probe or by PCR L!�3{ASIN0
analysis with primers. The 129/Sv Rhoh-/- mice were crossed with wild-type or p14 TCR �va�9�5/(�
(V 2V 8) transgenic mice on a C57BL/6J background to generate Rhoh-/- or V7�[Dvg:W
p14tg/+Rhoh-/- compound mice. Mice used were littermates derived from backcross /-8v]nR�B�
generations with an N of more than 2. The 129S6/SvEvTac-Rag2-/- mice were purchased �xQk�]��a1
from Taconic Animal Models. All animal experiments were approved by the Institutional �DS�i�zr4R
Animal Care and Use Committee of the Cincinnati Children's Hospital Research fP&F$"o8��
Foundation (Cincinnati, Ohio). jt�S+�y)�2
Antibodies and GST fusion proteins. q��4xB`��G
17 o!aKeM~|Es
Fluorescence-conjugated monoclonal antibodies to the following mouse antigens were GWM2l?�zOP
used for flow cytometry: CD4 (RM4-5), CD8 (53-6.7), CD25 (7D4), CD44 (IM7), TCR �LCyci1\�@
-chain (H57-597), TCR (GL3), TCR V 8, TCR V 5 (MR9-4), CD69 (H1.2F3), CD5 4���C�W
/�
(53-7.3), Gr-1 (RB6-8C5), Mac-1 (M1-70), NK1.1 (PK136), Thy1.2 (53-2.1), g�K-�:��t�
CD45R–B220 (RA3-6B2), IgM (R6-60.2), BrdU (3D4) and Ter119 (Ly-76; all from �}�)M$#%(�
Pharmingen). For immunoblot analyses, antibodies to the following were used: RhoH9 �!_�?<-f(�
(B4998), Zap70 phosphorylated at Y319 (17a), phosphorylated tyrosine (4G10) and Lat ��l(v$���+
(45; Pharmingen); hemagglutinin (3F10; Roche); -actin (AC-15; Sigma); CD3 ga�4 g�H>4
(6B10.2; Santa Cruz Biotechnology); and Lat phosphorylated at Y191 (3584), Zap70 K�e�&lGf"5
(99F2), phosphorylated p42-p44 (Thr202-Tyr204; 197G2) and p42-p44 (9102; Cell v@X�Q)95]F
Signaling Technology). Primary antibodies were detected with the secondary antibodies 2�8f�-8B��
horseradish peroxidase–conjugated goat anti-mouse (7076) or goat anti-rabbit (7074; both 9���(|[okB
Cell Signaling Technology), or donkey anti-rat (sc-2956; Santa Cruz Biotechnology) #Vs/1y`�()
using enhanced chemiluminescence detection (Cell Signaling Technology). GST fusion FT[oM<M\Xd
proteins were expressed in Escherichia coli BL21 (DE3) cells and were purified �Jj�fNH�
~
according to the manufacturer's recommendations (GE Healthcare Life Science). Purified �w�_�KGn17
GST fusion protein lysates were incubated for 1 h at 4 °C with glutathione–Sepharose 4B q�)��G�*�"
beads. Bead-bound GST fusion proteins were separated by SDS-PAGE and were 9(ZzwkD'>�
quantified by Coomassie blue staining. Rb#Z'1�D'G
GST precipitation assay. �O�.TFV.��
Jurkat cells were lysed in GST lysis buffer (50 mM Tris-HCl, pH 7.5, 150 mM NaCl, 10 �c5;YK�ON
mM MgCl2, 1% Nonidet-P40 and Complete Protease Inhibitors). Cell lysates were loaded Y@9L8�XNP>
onto columns of bead-bound GST fusion proteins. After columns were washed with GST vE�togkFA"
lysis buffer containing 150 mM and 200 mM NaCl, bound proteins were eluted with GST pr;<�n\�Y{
lysis buffer containing 400 mM NaCl and SDS sample buffer, sequentially. Eluted �� 7�z<!�2
proteins were detected by SDS-PAGE and Coomassie blue staining. Protein bands were �Yo|
H`m,�
identified with a Bruker Biflex III MALDI-TOF mass spectrometer (SpectroREADER; s�.=)p"pTd
Sequenom) and Protein Mass Fingerprinting Mascot search (Matrix Science). :��{_O�r'L
Subcellular fractionation. �~q4D�ePVE
Cells were lysed by brief sonication on ice in a buffer of 250 mM sucrose, 20 mM Tris, �eb9qg�.9Z
pH 7.8, 10 mM MgCl2, 1 mM EDTA, 1 mM Na3VO4, 10 mM NaF and Complete �2*K�0~ b`
Protease Inhibitors. Lysates were centrifuged to remove nuclei and debris (900g for 5 min "sT`Dh���r
at 4 °C). The P100 and S100 fractions were separated by centrifugation for 30 min at `�3p�e\�s�
100,000g. Membrane fractions were made soluble with MLB (Upstate) plus protease and m9#u��.�Q*
phosphatase inhibitors. After centrifugation for additional 30 min at 100,000g, the B��
susXW$
detergent-insoluble cytoskeleton-containing fraction was resolved by 0.5% SDS-PAGE. l�mH!I��)5
Assessment of Intracellular Calcium Concentration }^��`�{YD
