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Compassionate use of bevacizumab (Avastin) in children and young adults with !v?WyGbUg�
refractory or recurrent solid tumors. XF��Jz�\'{
Bevacizumab-induced transient remodeling of the vasculature in neuroblastoma ���7�Ug^aA
xenografts results in improved delivery and efficacy of systemically administered t��J9-8ZT*
chemotherapy. ����b�TJ l
Proteomics Approaches to the Systems Biology of Cardiovascular Diseases Q'R*a(�pm�
Pre- and post-natal treatment of hemophagocytic lymphohistiocytosis.
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Lack of early bevacizumab-related skeletal radiographic changes in children with p8|u�0/�;k
neuroblastoma. #�:�M <<gk
Interleukin-4 activates androgen receptor through CBP/p300 !6pE0(V^+4
Trisomy 8 in an allogeneic stem cell transplant recipient representative of a bY!1t}ALh�
donor-derived constitutional abnormality. T�V[@�!E a
Disruption of diacylglycerol metabolism impairs the induction of T cell anergy (��GB*+@��
T cell anergy is reversed by active Ras and is regulated by diacylglycerol kinase- D�WmViuZmL
High-dose conformal RT improves tumor control in patients with prostate cancer u3])�_oj=�
Vitamin D concentration does not affect the risk of prostate cancer j
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Liver resection with salvage transplantation for hepatocellular carcinoma `2P�vE4]%p
The impact of histopathologic diagnosis on the proper management of testis neoplasms o@�W:P�mKW
Prostate stem cell antigen is associated with diffuse-type gastric cancer dH_�g�:ocA
Multiple myeloma: high-risk immunophenotypes identified [��a!*m�<�
Increased c-kit expression predicts poor outcome in acute myeloid leukemia 2�9kR7[�k�
Global Analysis of the Meiotic Crossover Landscape �PsCr[\Ul�
Serum Response Factor Is Required for Sprouting Angiogenesis and Vascular Integrity y�_}jf,�b4
Integrin Trafficking Regulated by Rab21 Is Necessary for Cytokinesis oa2v/�P1`�
Reduced Translocation of Nascent Prion Protein During ER Stress Contributes to L����6�n<h
Neurodegeneration _t.U�b��:�
Effects of oral niacin on endothelial dysfunction in patients with coronary artery disease: (c|Ry��[$|
Results of the randomized, double-blind, placebo-controlled INEF study. W
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Global experiences with vardenafil in men with erectile dysfunction and underlying 09sdt;V �Q
conditions. E-��"b":@:
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Noninvasive cardiac imaging: implications for risk assessment in adolescents and young E)]RQ~jY�?
adults. B0$.oa�vC�
Transforming growth factor beta1 T29C gene polymorphism and hypertension: <0���!)}O�
Relationship with cardiovascular and renal damage. ��E�%vT(Kz
A comparison of hormone therapies on the urinary excretion of prostacyclin and �d6+{^v�$#
thromboxane A2. ��%W�,V~kb
Repair of an infected aortic aneurysm using an aortic allograft and a venous autograft: :�,1�kSM%r
Report of a case. Q/��^�a(��
Circulating Leptin and Stress-induced Cardiovascular Activity in Humans. !B:wzb���_
Effects of aspirin dose on ischaemic events and bleeding after percutaneous coronary Rn5{s3?F~2
intervention: insights from the PCI-CURE study. F�|^tRL�-�
Long-term cardiovascular outcomes following ischemic heart disease in patients with and �U2
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without peripheral vascular disease. XG;Dj<�Dm�
Reduced renal function and sleep-disordered breathing in community-dwelling elderly f&8�8��N<)
men. GRj#1OqL�
Intracoronary pharmacotherapy in the management of coronary microvascular @lTd,�V�5f
dysfunction. bm#/ KT_�8
Inhibition of platelet aggregation by combined therapy with aspirin and cilostazol after PI�ZK*L�op
off-pump coronary artery bypass surgery. #�s�3�R4@{
Inhibition of CCR2 Ameliorates Insulin Resistance and Hepatic Steatosis in db/db Mice :�BpXi|n;�
Abstract 要求简洁,连贯 MVOWJaT(Aq
The acquisition of metastatic ability by tumor cells is considered a late event in the �/j�;�HM[�
evolution of malignant tumors. We report that untransformed mouse mammary cells that #v�}pn2g%>
have been engineered to express the inducible oncogenic transgenes MYC and KrasD12, or �,�B,:$G<�
polyoma middle T, and introduced into the systemic circulation of a mouse can bypass v#b(��
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transformation at the primary site and develop into metastatic pulmonary lesions upon `���<I�aQY
immediate or delayed oncogene induction. Therefore, previously untransformed '-M9�v3itC
mammary cells may establish residence in the lung once they have entered the �~R
���C\
bloodstream and may assume malignant growth upon oncogene activation. Mammary �"eZ~]m}L0
cells lacking oncogenic transgenes displayed a similar capacity for long-term residence in �\CVr�Ln;}
the lungs but did not form ectopic tumors. �KSxZ��4�Y
Almost two decades after CFTR was identified as the gene responsible for cystic fibrosis �Z^6qx�ZJ7
(CF), we still lack answers to many questions about the pathogenesis of the disease, and it ]3�I@5�}5%
remains incurable. Mice with a disrupted CFTR gene have greatly facilitated CF studies, �rB}2F�*eT
but the mutant mice do not develop the characteristic manifestations of human CF, m�a�e@�
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including abnormalities of the pancreas, lung, intestine, liver, and other organs. Because $n��_ax\15
pigs share many anatomical and physiological features with humans, we generated pigs Z:.*f��s�5
with a targeted disruption of both CFTR alleles. Newborn pigs lacking CFTR exhibited �RKD$'UW�X
defective chloride transport and developed meconium ileus, exocrine pancreatic <�Xb$YB-c�
destruction, and focal biliary cirrhosis, replicating abnormalities seen in newborn humans jYE
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3 iE�,/x^&,&
with CF. The pig model may provide opportunities to address persistent questions about k293���wS�
CF pathogenesis and accelerate discovery of strategies for prevention and treatment. M=#g_��*d�
Variable lymphocyte receptors (VLRs) rather than antibodies play the primary role in Q(��/F7�"m
recognition of antigens in the adaptive immune system of jawless vertebrates. r;SOAuc�X
Combinatorial assembly of leucine-rich repeat (LRR) gene segments achieves the �� 2��c%b�
required repertoire for antigen recognition. We have determined a crystal structure for a &�F�Y7
D<
VLR-antigen complex, VLR RBC36 in complex with the H-antigen trisaccharide from :aWC6"ik-W
human blood type O erythrocytes, at 1.67 angstrom resolution. RBC36 binds the �)Ag{S[yZ�
H-trisaccharide on the concave surface of the LRR modules of the solenoid structure e~P�Ai8B�5
where three key hydrophilic residues, multiple van der Waals interactions, and the highly *nlD�N4Y[�
variable insert of the carboxyl-terminal LRR module determine antigen recognition and �} bm ^`QY
specificity. The concave surface assembled from the most highly variable regions of the �B�oP,Mp�F
LRRs, along with diversity in the sequence and length of the highly variable insert, can M+-1/vR *@
account for the recognition of diverse antigens by VLRs. m4,�inA:�o
A 51-year-old man with a diagnosis of myelodysplasia and non-Hodgkin's lymphoma +%?�\#E�QJ
underwent an unmatched allogenic bone marrow transplantation and was treated \
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posttransplant with chronic immunosuppressive medication. Eight months following �l^�R1XBP�
transplantation, he presented with progressive dysarthria, cognitive and visual decline. ].
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Evaluation included brain magnetic resonance (MR) imaging demonstrating multifocal �J
Mm'J�K?
areas of increased T2 and FLAIR (fluid attenuated inversion recovery) signals involving C~���R�,�,
the left frontal, parietal, and occipital lobes. The MR lesions demonstrated diffuse Hle�M�zykF
increased signal on DWI (diffusion-weighted images) and normal to low signal on ADC V?-Sv�QIk1
(apparent diffusion coefficients). Contrast-enhanced T1 images were unremarkable. ��>Do�P2�]
Lumbar puncture revealed a mild elevation in cerebrospinal fluid (CSF) protein. CSF l�i9>�zjz�
PCR assay for viral DNA fragments were negative on two occasions. Serum serology for MR/gLm
(8(
HIV was negative as well. A brain biopsy was subsequently performed. The clinical and pZ5eG�A=��
neuroimaging differential diagnoses as well as neuropathologic correlation are presented. �7uq^TO>9f
In vitro-generated mesenchymal stem cells (MSCs) initially attracted interest for their #]z�_p�p�:
ability to undergo differentiation toward cells of different lineages. =`.OKU�A�n
These results suggested that ZiC~8p�_f�
However, there are still obstacles in cBQ+`DXn5c
The major challenge for successful drug development is identifying delivery strategies g[(Eh?]Sc�
that can be translated to the clinic. -;iCe7|Twf
This review will discuss progress in developing and testing small RNAi-based drugs and -`,�F��e�3
potential obstacles. �kHd`k�.nW
This review highlights what '�M,O(utGv
In addition, there are indications that /om�m���M�
Proper consideration of all of these issues will be necessary in d$�:LUx�M#
These studies provide 4�P^CqD�&i
This paper presents the potential applications and the hurdles facing anti-HCV siRNA k1~? �}+<e
drugs. >*�W�T[�UU
The present review provides insight into the feasible therapeutic strategies of siRNA 1!A��fq}|
technology, and its potential for silencing genes associated with HCV disease. @0-�vf>e3-
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A basic problem in the design of xx is presented by the choice of a xx rate for the 6Cgc-KN�bk
measurement of experimental variables.
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This paper examines a new measure of xx in xx based on fuzzy mathematics which ��ftD(ed��
overcomes the difficulties found in other xx measures. ��
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This paper describes a system for the analysis of the xx. ^J)0i_RS��
The method involves the construction of xx from fuzzy relations. �m^�>v~Q~~
The procedure is useful in analyzing how groups reach a decision. dZC��nQ�IS
The technique used is to employ a newly developed and versatile xx algorithms. L�vNulME�K
The usefulness of xx is also considered. #Ve@D�@d�[
A brief methodology used in xx is discussed. ]���E^)d|_
The analysis is useful in xx and xx problem. d fSj�= 4�
A model is developed for a xx analysis using fuzzy matrices. OJD!�A�r8Q
Algorithms to combine these estimates and produce a xx are presented and justified. }z5u�^�_-m
The use of the method is discussed and an example is given. 5
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Results of an experimental applications of this xx analysis procedure are given to }J� �$\<ZT
illustrate the proposed technique. wY3|�5kbDj
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achieving a hierarchical system of objectives are evaluated. !,�R=6b$E5
The main emphasis is placed on the problem of xx �>�fzFNcO*
Our proposed model is verified through experimental study. D��B(!*6#?
The experimental results reveal interesting examples of fuzzy phases of : xx,xx ^O,r8K{�1n
The compatibility of a project in terms of cost, and xx are likewise represented by *d9RD~��Ee
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requiring mechanical ventilation, which greatly increases mortality KxDp+]�N]
The cause of respiratory failure in patients with AKI is incompletely understood ��nO�#x��"
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as the liver, gut, and hind limb }s[`T� ���
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Polyphenolic compounds are vasodilators and help to lower the risk of cardiovascular �/4@
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diseases. �D c;k)z�=
Taken together, our novel findings suggest that the EDR induced by the strawberry 4c[�/%e:\-
extract was mediated by activation of the PI3 kinase/Akt signaling pathway, resulting in Cy��)N hgz
phosphorylation of eNOS. "YW�Z&_n**
Objective / Goal / Purpose @DF7�j|]tV
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knowledge in the area of manual handling of loads, and to provide intelligent, y#th&YC_b�
computer;aided instruction for xxx. -�y{(h%�
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fuzzy data: xx. �!��|��UX4
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deiodinase activity due to a mutation in SBP-2 Cb�C�[aVA=
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cellular and molecular aspects of local control of thyroid hormone signaling provided by <�
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fit well with this narrowly defined model. They tend to span broad activities and require ��b*h:e.q�
consideration of multiple aspects. �.j�P|�b~�
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real;world problems and data, we have to pay attention to the problems of xx and xx. q�3v5g�z^t
MATERIALS AND METHODS ��8yOhKEPX
Materials fO�#nSB/
8
Chemicals were purchased from Sigma (St Louis, MO), if not stated otherwise. #Ddo` �>`&
Experiments were conducted in accordance with the NIH Guidelines for the Care and Use 58mpW��`�Q
of Laboratory Animals. ���D\�J.6W
CsA, EGF, PD98059, U0126, AG1478, Wortmannin, and LY294002 were from 6e.l#
c!1}
Calbiochem (San Diego, CA, USA). Anti-ERK1/2 and anti-Ras were from Transduction |�G/�)�<1P
Laboratories (Franklin Lakes, NJ, USA). Anti-phospho Raf-1 (Ser259), anti-phospho �S�&l� [z,
Raf-1 (Ser338), anti-phospho PKB/Akt (Ser473), anti-PKB, anti-phospho EGFR (Tyr1068), O\=Zo9(NHF
anti-phospho ERK1/2 (Thr202/Tyr204), anti-PI3K 110 , anti-p53, and anti-phospho C^_m>H3�b�
MEK1/2 (Ser217/221) were from Cell Signalling (Danvers, MA, USA). Anti-MEK and plr3&T~,&S
anti-Raf-1 (C12) were from Santa Cruz (Santa cruz, CA, USA). Apigenin and all other L|b[6[XTHL
reagents were from Sigma (Saint Louis, MO, USA). p,(W?.ZDN?
Animal Ed-3-vJej6
Eight- to ten-week-old male C57BL/6 mice (wild-type) and IL-6-deficient mice ]�TtI�D4qL
backcrossed over eight generations on a C57BL/6 background were used e�6 <9`X�g
Mice were maintained on a standard diet and water was made freely available. 5V/]��7>b1
All experiments were conducted with adherence to the NIH Guide for the Care and Use @0tX�,Z
�9
of Laboratory Animals. ;jP�iD`Kyv
The animal protocol was approved by the Animal Care and Use Committee of the e�qO�T@�~H
University of Colorado 9R-���2\D]
Three surgical procedures were performed as described previously:5 (1) sham operation, ~`$P-^u88X
(2) ischemic AKI, and (3) bilateral nephrectomy. ,5T1QWn^�f
The abdomen was closed in one layer. �@S5HMJ�2=
Sham surgery consisted of the same procedure except that clamps were not applied. j�]-�_k�jt
9 �-M T1q�qi
For bilateral nephrectomy, renal pedicles were tied off with suture and then cut distally. ��Pv���)^L
The ureters were pinched off with forceps and the kidneys removed. B��T3yrq�9
Serum was collected as described previously.5 Blood urea nitrogen and creatinine were w|0�:0Rc~u
measured using an autoanalyzer (Beckman Instruments, Fullerton, CA, USA). !`W0�;0'Zg
Serum IL-6 was measured by ELISA according to assay instructions (R&D Systems, F�f
=%�eg]
Minneapolis, MN, USA). �7G��Er�h,
Five-micrometer sections of paraffin-embedded lung tissue were stained with �VH+3o?nrT
hematoxylin and eosin using standard protocols. Neutrophils were counted on the basis of w��7q6��v>
morphological criteria; at least 50 high-powered fields ( 40) were counted per slide. c7[Ba\Cr4h
Frozen lung was prepared for ELISA as described previously.5 Supernatants were xBf->o �S?
analyzed for protein content using a Bio-Rad DC protein assay kit (Hercules, CA, USA). Qs#;sy
W@~
KC and MIP-2 were determined by ELISA (R&D Systems, Minneapolis, MN, USA). s �b��R*[2
One-fourth lung was used to determine MPO activity as described previously. |]Hr"saO0�
Frozen lung was homogenized in radioimmunoprecipitation assay buffer with protease �sK/ymEfRv
inhibitor; western blotting was performed as described previously.49 Goat anti-murine U�V�{})T*s
ICAM-1 polyclonal antibody (R&D Systems, Minneapolis, MN, USA; 1:2000) or rat 6iH�Y{WcDj
anti-murine VCAM-1 monoclonal antibody (R&D Systems; 1:1000) were used. >�'WTVj�`
A total of 20 g anti-IL-6 antibody vs IgG control (eBioscience, San Diego, CA, USA) ��Wy�M�2h�
was administered to wild-type mice by tail vein injection 1 h before surgery, �'*�@��=SM
intraperitoneally at the time of clamp removal (ischemic AKI) or nephrectomy (bilateral *mY�Gs� )|
nephrectomy) and intraperitoneally 1 h following surgery (60 g total). ,C��_MB�1u
Experimental groups O�JM2t`}_t
STZ-induced diabetic rats, a model of partial type I diabetes: SD rats received a single Are0Nj&?��
intraperitoneal injection of freshly prepared STZ (65 mg kg-1 body weight, dissolved in j+g�h*�\:q
100 mmol l-1 citric acid, pH 4.5), and confirmed 2 days later by PP blood glucose m*i,|{�UZ�
(>250 mg dl-1). ��&h7
�n>q
CTR rats: Vehicle-injected SD rats after 2 to 7 days, 14 to 30 days, and 90 days served as q& K��NK��
CTR for the 2 and 7 days STZ, the 14 and 30 days STZ, and for the 90 days STZ, S&'s�/jB��
respectively. Znh�;#�%n|
Insulin treatment in STZ: Glc was normalized in seven animals during 12–14 days of 9U )9u["DH
STZ by subcutaneous insulin implants (2U day-1; Lin Shin Canada, Ontario, Canada). �)!�G� �10
Cell Culture nhZ/^��`Y<
Immortalized cells from the convoluted portion of mouse kidney proximal tubule /_8�nZV�u�
PKSV-PCT cells (PCT3 clone) were cultured in a medium A (DMEM/Ham's F12 (1:1, rH\�o�FCzC
v/v), 20 mM HEPES, 2 mM L-glutamine, 12.5 mM D-glucose, 60 nM sodium selenite, *UG?I|l|I�
5 g ml-1 transferrin, 50 nM dexamethasone, 100 U ml-1 penicillin, and 100 g ml-1 NH=@[t)�P,
streptomycin), supplemented with 2% fetal bovine serum, 5 g ml-1 insulin, 10 ng ml-1 -?I�F'5�z�
EGF, and 1 nM triiodothyronine at 37°C in a 95:5 air/CO2 water-saturated atmosphere. x>A[~s"|�N
For all experiments, cells were seeded at 0.2 106 cells/ml and after 24 h with complete !#e+�!h�@�
medium cells were starved for 16 h in medium A supplemented with 0.1% fetal bovine D})12qB;u9
10 &#���.>-D{
serum but not insulin, EGF, or triiodothyronine. CsA was dissolved in ethanol and all the sP=^5�K`�g
pharmacological inhibitors were in DMSO. In all cases, controls were carried out with mG�F�)Ot R
cells treated with the corresponding vehicle alone. After treatments, cells were washed qc3,�/JO1�
twice with cold phosphate-buffered saline (PBS) and harvested with lysis buffer as in 0|�=y#`;,Z
Llorens et al �I@#IX�H?6
Cell viability Z��,~@_�;F
After treatments, PCT3 cells were harvested and washed twice with cold PBS, and the z|(<Co�8#.
viable cells were counted with Trypan Blue Dye (Gibco-Life Technologies, Grand Island, Wu8zK=�Ve(
NY, USA) in a Neubauer chamber. Living cells exclude the dye, whereas dead cells will J�v�]$@�>#
take up the blue dye. For Hoechst staining, cells seeded in six-well dishes were washed hx:^xW@r4P
twice with PBS and fixed for 15 min with 4% paraformaldehyde at room temperature. �A.$P1z�wC
Then, cells were washed twice again with PBS and stained with Hoescht (5 g ml-1 in 2)�QZYgf�h
PBS) for 5 min. KAu>U�3�\/
Western blots/ Immunoblot 2�nL*^hhh�
The protein content of cellular extracts was quantified by the Bradford assay.44 Wdj|�
�RKw
Twenty-five microgram of total cell extract protein was run on SDS-polyacrylamide gel �$�) qL=kR
electrophoresis gels, transferred onto polyvinylidene difluoride membranes, and
u��6MU
@?
incubated with the corresponding antibodies. The membranes were developed with the E9���@Sc>e
enhanced chemiluminescence method (Pierce, Rockford, IL, USA). I"K�o��sSs
Supernatants of growing or growth-arrested cells were centrifugated for 5 min at 10 000 g. �Q�j|t�D+<
The cells were lysed as described. The proteins from supernatant and cell lysates were {
��qC�F�d
concentrated using heparin sepharose. The heparin sepharose was washed four times with K�<p
�Z*l�
phosphate-buffered saline containing protease inhibitors, dissolved in phosphate-buffered y*=I�pdj��
saline/protease inhibitor and incubated with 500 g protein over night at 4°C. The vCOtE�D�*<
complexes were washed with phosphate-buffered saline/protease inhibitor and the oP:R�1��<�
proteins were eluated with 100 l Laemmli buffer without bromophenol blue (10 min ?_T[�]I�'�
95°C). A 30 l probe was loaded in each lane and western blot analysis was performed as \,lIPA/�L�
described, using a polyclonal antibody against CCN3 (K19M), which recognizes a ,<s:*
���k
C-terminal 19-aminoacid peptide of human CCN3. As a positive control, a supernatant |nqN95'u+]
from adrenocortical cell cultures, which are known to secrete CCN3, was used. 3'��SN�0VL
Cells were lysed in 0.5% (volume/volume) Triton X-100 lysis buffer and immunoblot ��M.EL^;r�
analysis was done as described43. Immunoprecipitation with anti-CrkL or control rabbit K����@:t�6
antiserum was done as described44. Antibodies to the following were used: �pP#
|:� %
phosphorylated Erk (910L; Cell Signaling); phosphorylated Jnk (V7932; Promega); Erk Eb5BJ-XeS^
(13-6200; Zymed); Jnk1 (sc-474), H-Ras (sc-35), C3G (sc-869), CrkL (sc-319), OO,EUOh-T:
RasGRP1 (sc-8430) and DGK- (sc-8722; all from Santa Cruz Biotechnologies); and VS_I'SPPIc
DGK- (a gift from H. Kanoh, Sapporo Medical University, Sapporo, Japan). Images �]AN%#1++U
were scanned, followed by densitometry analysis with UN-SCAN-IT software (Silk G�BT219Z@8
Scientific). (�io[�O?te
11 ,�z�Z@QW�5
Purified splenic T cells were stimulated for various times with 5 g/ml of anti-CD3 z2#k�/3%o=
(500A2; BD Pharmingen) and were lysed in 1% Nonidet P-40 lysis buffer (1% @,L�U!#y�(
(volume/volume) Nonidet-40, 150 mM NaCl and 50 mM Tris, pH 7.4) with protease �]x%�sX|Rj
inhibitors. Proteins were resolved by SDS-PAGE and were transferred to a Trans-Blot �-av=5h�m�
Nitrocellulose membrane (Bio-Rad Laboratories); membranes were probed with )d|s$l$�?7
antibodies specific to phosphorylated Erk (91015; Cell Signal Technology) and �,)V�AKrSg
phospholipase C- 1 (05-163; Upstate Biotechnology). Membranes were stripped and J�c
f�G�e4
were reprobed for analysis of total Erk (SC-16982; Santa Cruz Biotechnology). Activated �oqg +�<m�
Ras in cell lysates was determined by glutathione S-transferase–Raf—Ras-binding �d\8j!F�^=
domain precipitation assay as described ~c*kS E�2X
Immunofluorescence microscopy. Rv.�IHSQUo
Analysis of protein localization in 2C T cell–P815.B71 cell conjugates was done as Qc�jsQTAbk
described29. P815.B71 cells were labeled with CMAC (7-amino-4-chloromethylcoumarin) NiRb�:��F-
Cell-Tracker Blue (Molecular Probes) and were mixed with equal numbers of anergic or D'^UZZlI^I
in vitro–primed 2C Rag2-/- T cells. After approximately 8 min, cells were fixed, were �
�sN) xNz
made permeable and were stained with anti-GRP1 and anti-talin (Santa Cruz SQ'%a�-Mct
Biotechnologies) and with species-specific secondary antibodies conjugated to Q�B���;TQZ
fluorescein isothiocyanate or phycoerythrin, respectively. Samples were analyzed with a ~��3%�aEj�
Zeiss Axiovert 100 microscope, and 15 conjugates were typically assigned scores. aEun� *V^,
Slidebook software (Intelligent Imaging Innovations) was used for image capture and 1{1mL�-I�;
deconvolution analysis. ImageJ 1.36b software (US National Institutes of Health) was #nmh=G?\Sm
used for quantification of pixel intensity. �*nv���^�s
Measurement of ROS generation ��lAGnt
Yv
The assay is based on the incorporation of 2',7'-dichlorofluorescein diacetate into the cell. 0o�q��O��X
H2O2 and peroxidases are able to oxidize the cleaved DCFH to DCF, which is highly 7$��8DMBqq
fluorescent at 530 nm. To measure CsA-induced ROS generation, cells were washed IIF� <Zkpb
twice with PBS, and fresh medium containing 20 M 2',7'-dichlorofluorescein diacetate C���Bz=-Xr
was added to previously treated cells. After 30 min cells were washed again, tripsinized, kL��<HG�Qt
and resuspended with cold PBS. Fluorescence was measure by flow cytometry on a kv2� �H3O�
FACScan flow cytometer. g[�\8s~g,�
Raf-1 activity ]��L�MtZUz
Raf-1 immunoprecipitation and kinase assay were performed as described previously.45 �3�T�[zieX
Immunoprecipitated Raf was incubated for 30 min at 30°C with 0.8 mM ATP, 10 g ml-1 �b'�vIX<
g
GST-MEK, and 100 g ml-1 GST-ERK2. An aliquot of the supernatant was used for Vl'rO
_�?t
ERK2 activity assays using 0.5 mg ml-1 myelin basic protein and 0.1 mM [ -32P] ATP �:�?>yi�7w
(400 c.p.m. pmol-1). After 15 min incubation at 30°C, 12 l of 5 Laemmli loading - rI4_D�l�
buffer was added to the tubes and the mixture analyzed by SDS-polyacrylamide gel ���Z4m+GFY
electrophoresis. Radiolabeled bands were quantified in a PhosphoImager. #RKd�>ig%
12 LC��e6](�Z
Semiquantitative RT-PCR. 2�tQ?=V(Di
Total RNA was isolated from freshly isolated thymocytes. Then, cDNA was prepared _��:��Jma
with the M-MuLV reverse transcriptase and random primers according to the S�%w��d�Xe
manufacturer's recommendations (New England Biolabs). Semiquantitative PCR analysis x�1"�8K���
of Tcrb VDJC (where 'C' is the constant region) and Cd3e cDNA was done as described51. �N�Ff`���V
[32P]dCTP (GE Healthcare Life Science) was incorporated into PCR products for 6=*n$l�#�}
semiquantitative detection by autoradiography. #I�J6pg�>K
Real-time quantitative RT-PCR N�L'(/|)��
Total RNA was isolated from HMC or rat mesangial cells using the Invisorb Spin �^S(�QvoaQ
Cell-RNA Mini Kit (Invitek, Berlin, Germany) or from isolated glomeruli using the .}�E�@�7^X
RNeasy Mini Kit (Qiagen, Hilden, Germany). RNA purity determination, cDNA )q[Wzx_ j<
synthesis, and RT-PCR were performed as described.16 Primer sequences are listed in �aPX'�CG4m
Table 2. Glyceraldehyde-3-phosphate dehydrogenase cDNA amplification was used as an �hE�'>8�{�
internal standard. �]@CXUa,>a
Total RNA was isolated from the frozen kidneys as described by Chomczynski and ?�uW}�
XAi
Sacchi47 and quantified by a photometer. One microgram of the resulting RNA was used Oe;1f#`�5�
for reverse transcriptase (RT)-PCR. The cDNA was synthesized by MMLV reverse Ci�2*��5n<
transcriptase (Superscript-Invitrogen, Carlsbad, CA, USA). For quantification of renin /�XdLdA!v
mRNA expression (sense: 5'-ATGAAGGGGGTGTCTGTGGGGTC-3', antisense:
=p dL�h
5'-ATGCGGGGAGGGTGGGCACCTG-3'), real-time RT-PCR was performed using a 1k{H�,p�7�
Light Cycler Instrument (Roche Diagnostics Corp., Basel, Suisse) and the QuantiTect *T.V�5FB0S
SYBR Green PCR kit (Qiagen, Hilden, Germany), with GAPDH (sense: �hW\'E�J�
5'-TTCATTGACCTCAACTACAT-3', antisense: 5'-GAGGGGCCATCCACAGTCTT-3') 7���Q~$&�G
as a control. PCR was run for 30 cycles with 15 s per 95°C denaturation, 20 s/58°C 3�~LNz8Z�*
annealing and 20 s/72°C elongation. To verify the accuracy of the amplicon, a melting -oY8]HrXfK
curve analysis was done after amplification.Total renin mRNA content per kidney was )�"6�3g��
calculated from the yield of RNA extracted from the whole kidneys times the renin �8<���J3Xe
mRNA estimate obtained from the defined amount of RNA used for RT-PCR real time ]1I-�e2Q-J
measurement. For the RT-PCR real-time measurements, a pool of RNA from adult mouse yv�nv�I�y�
kidneys was generated, which served as standard for all RT-PCR runs. Thus, all renin ;Q[E>j�?w=
mRNA levels for the developing kidneys were estimated relative to the levels in adult BG6Lky/omz
kidneys. !yz3:Yz
�u
In vitro anergy assay. EH'eyC-�B<
Wild-type, Dgka-/- and Dgkz-/- splenocytes were stained with 5 M CFSE, were �]jR-<l8I-
stimulated for 72 h with anti-CD3 (1 g/ml; 2C11) along with CTLA-4–Fc (5 g/ml), {#&D=7��LP
were stained with allophycocyanin-conjugated anti-CD4 and were analyzed by flow 0�QEcJ]Qb8
cytometry. Cell division was assessed by CFSE dilution after gating on live CD4+ cells. 'H�u+8,xA
Alternatively, cells were stimulated for 72 h and were pulsed with 1 Ci/well of �MYVb �!�
[3H]thymidine for the final 8 h of stimulation, and proliferation was assessed by tritium �WY26�Iq@C
incorporation with a scintillation counter. For restimulation analyses, cells were 4�6H�@z�=5
13 �}T5�3y6J#
prestimulated with anti-CD3 plus CTLA-4–Fc, then after 72 h, CD4+ cells were purified ZR8y
9mx2"
by negative selection (with fluorescein isothiocyanate–conjugated anti-CD8, anti-B220 �!�.O�;S�G
(RA3-6B2; BD Pharmingen), anti-DX5 and anti-CD11b (M1/70; BD Pharmingen), 2Ic�)]6z
R
followed by depletion with anti–fluorescein isothiocyanate magnetic beads) and were c�q/@ng�*o
allowed to 'rest' overnight at 37 °C. Live cells were then counted by Trypan blue t�n�|H~iF{
exclusion, and equivalent numbers of live cells were dropped onto monolayers of bone D<[kbt�5^7
marrow–derived macrophages coated with anti-CD3 (1 g/ml) and anti-CD28 (0.5 �zJOyr"B'8
g/ml). After 24 h, supernatants were collected and IL-2 was quantified by ELISA 0��C��yus�
according to the manufacturer's protocol (R&D Systems). uTy00�`�1�
Three-dimensional reconstruction �-y/Y%�]%0
Serial sections of kidney specimens were fixed and stained for renin and for SMA as w~n+�hh�MF
described above. Digitalization of the serial slices was performed using an AxioCam V�! .�I��>
MRm camera (Zeiss, Jena, Germany) mounted on an Axiovert200M microscope (Zeiss) tN����AmA�
with fluorescence filters for renin and SMA (TRITC: filter set 43: Cy2: filter set 38 HE; u�Y3?�(f�#
Zeiss). After acquisition, a stack of equal-sized images was built using the graphic tool Q0L1!}w
��
ImageJ (Wayne Rasband, NIH, Bethesda, MD, USA). The equalized data were then I1p{(f��J�
imported into the Amira 4.1 visualization software (Mercury Computer Systems Inc., U�UvR�>5@n
Chelmsford, MA, USA) on a Dell Precision 690 computer system (Dell, Frankfurt, 6hH�MxS^o�
Germany), and subsequently split into the renin and SMA channels. After this step, the w=~X��6[+3
renin and SMA channels were aligned. In the segmentation step, the SMA and renin 2TQ�<XHA�\
data sets served as a scaffold and were spanned manually or automatically using }�3�-��`e3
grayscale values. Matrixes, volume surfaces, and statistics were generated from these j(c;�r���>
segments. `mqu��Gk|)
Restimulation assay after in vivo immunization. EI�OP+9zP�
For analysis of T cell priming in vivo, CD4+ T cells were collected from naive, primed or �jT�qE�V
(
tolerized recipient mice on day 15 after immunization. Proliferative responses were ��(7X^�z&2
measured by culture for 72 h of CD4+ T cells (3 106 cells/ml) with irradiated (3,000 rads) 1��.�nY�T*
APCs (10 106 cells/ml) and OVA(323–339). The number of KJ1-26+ cells for each d\t�A1&k71
group of recipient mice was determined by flow cytometry and proliferation was 3+!��G�9T!
normalized to the number of input KJ1-26+ cells. Supernatants were collected from plates /@",�5U�#�
and cytokine concentrations were measured by ELISA. ua�o#=]�?)
Flow cytometry. �{=+�'3�p�
For analysis of surface antigen expression, mAb to CD4 (JK1.5; eBioscience) and mAb f;�b�f�R&v
KJ1-26 (KJ-126; Caltag) were used. For intracellular IL-2 staining, T cells were :]�8�!G- Z
restimulated for 24 h in vitro with OVA(323–339) in the presence of APCs as described yz%o�?�%�@
above. Brefeldin A (eBioscience) was added for the last 6 h of the culture. Cells were �&#'�.�I0n
collected and were stained with allophycocyanin-conjugated mAb to CD4 and fluorescein x,
'KI?TyQ
isothiocyanate–conjugated mAb KJ1-26. Then, cells were fixed, were made permeable eX'V
#K�#C
and were stained with antibody to IL-2 (clone JES6-5H4; eBioscience) according to the �S�Yg�kY�R
manufacturer's instructions. ZD4:'m`�T/
14 m��wF{z.t"
TH1 cells transduced with adenovirus vector encoding GFP were analyzed with a S]�gV!�Q4%
FACScan (BD Biosciences). A total of 1 104 events were acquired, and data were ?p>m�;�Aq�
analyzed with CellQuest software (BD Biosciences). �uFf�k�!��
Splenic and lymph node samples depleted of thymocytes and red blood cells were stained I@(�3~ A�b
with fluorescence-conjugated anti-CD3 (2C11), anti-CD4 (GK15), anti-CD8 (53-6.7), $/�Llzpvny
anti-CD25 (7D4) and anti-CD44 (552407; all from BD Pharmingen). A three-color M|UCV_�omN
FACScan (Becton Dickinson) was used for flow cytometry, and data were analyzed with HzAw
�rC��
FlowJo 4.6 (TreeStar). �P��o�\�d!
A FACSCalibur (Becton Dickinson) was used for flow cytometry. Human cells from `F_R J.g*p
transplanted NOD-SCID mice were assessed with phycoerythrin–cyanin 5–conjugated +[[^W;<.l
anti–human CD45 and phycoerythrin-conjugated anti-CD19, anti-CD33, anti-CD36 and eo&G@zwN��
anti–glycophorin A (Becton Dickinson). EGFP fluorescence was detected with channel m�=60a@�o]
FL1 calibrated to the fluorescein isothiocyanate emission profile. During quadrant
z#6(PZC�}
analysis, only fluorescence excluding more than 99% of isotypic control events was m-Q�y�6"eW
considered specific. Cell Quest Pro software (Becton Dickinson) and FlowJo (Tree Star) Am >b�7�Z!
were used for data acquisition and analysis. K�#R|G�Ewr
Mammalian expression plasmids and transfection. 2F/oW�t|w?
For generation of the plasmid expressing Smad3 shRNA, the following specific ##s�:��Ww
oligonucleotides were used: upper, s�l)]yCD|5
5'-GATCCACCTGAGTGAAGATGGAGATTCAAGAGATCTCCATCTTCACTCAGG (XV+a�Q�\A
TTTTTTTACGCGTG-3'; lower, p &����i+i
3'-AATTCACGCGTAAAAAAACCTGAGTGAAGATGGAGATCTCTTGAATCTCCA ;A�o`yC2(v
TCTTCACTCAGGTG-5'. These were cloned under control of the U6 promoter into the S)�`��@)sr
pSIREN-DNR-DsRed expression vector (Clontech, BD). Vector expressing shRNA VwT&A9&{�8
specific for luciferase served as a control. Smad3-Tm was subcloned into the _D�8�:p>=�
pIRES2-EGFP vector (Clontech, BD); empty vector served as a control. Purified �R�G_�6&
A
DO11.10 or DO11.10p27 T cells were transfected with plasmids by nucleofection with �}-�p�-(��
the Amaxa nucleofection apparatus, according to the manufacturer's instructions (Mouse !j9(%
,P�R
T Cell Nucleofector Kit Amaxa Biosytems). Purified T cells were suspended in �Q��a"
4^s
nucleofector solution (3 106 cells/100 l) and were mixed with 3 g of plasmid. �&
z5:v-G?
Samples were transferred into cuvettes, were transfected with nucleofector program X-01 �fjm�3X$tR
and were then immediately transferred into 12-well plates and were cultured in l7(p~+o?h>
nucleofector medium for 3 h. Then, cells were collected and counted and were ��27Vx<W��
immediately transferred into syngeneic recipient mice (3 106 cells per mouse). At 3 h D 7�5;Y�;E
after adoptive transfer, mice were given priming or tolerizing treatment in vivo according ,8stEp9~h]
to the standard protocol described above. Lymphocytes were isolated from draining �~�oRT@�E�
lymph nodes at day 5 of the treatment, CD4+ T cells were purified and transfection wi�f1|!�aL
efficiency was assessed by flow cytometry. The range of transfection efficiency was -5@hU8B'�a
69–75% (Supplementary Fig. 4 online). Smad3-knockdown and control-knockdown *nwH1�F�jH
DO11.10 cells and DO11.10 cells transfected with Smad3-Tm and vector control were ��-'�Z�-8�
selected by cell sorting. The resulting CD4+ T cells (2 106 cells/ml) were restimulated � k.\4<�}�
with OVA(323–339) (5 g/ml) in the presence of irradiated APCs in vitro. )�#,a'�~w�
15 -�$�`q��:j
Luciferase assays. �2�nS�K}�q
CAR IL-2–Luc TH1 clones were transduced with vectors, were stimulated for 20 h and c&�"1Z/�tR
were resuspended in serum-free DMEM in luminometer cuvettes (BD Biosciences). An jgBJs^JgYG
equal volume of Bright-Glo luciferase assay reagent (Promega) was added to each sample, H�^g&e�$d0
followed by thorough mixing. After 2 min, samples were analyzed with a monolight 2010 7/dp_I}�cO
Luminometer (BD Biosciences). ����|p�E
~
Analysis of cell divisions in vivo. �����;ih;8
Purified T cells from DO11.10 and DO11.10p27 mice (10 106 cells/ml) were labeled �5�Z13s���
for 30 min at 37 °C with the intracellular fluorescent dye CFSE (5 M 5(and G�Q*o�r>R1
6)-carboxyfluorescein succunimidyl ester; Molecular Probes). Then, cells were washed ^%qQ�)>I=j
twice with cold RPMI 1640 medium containing 10% FCS, were resuspended in PBS and \4uj!LgTb
were transferred intravenously into BALB/c mice (5 106 cells per mouse). Syngeneic n�gz�QVaB9
hosts were left untreated (naive) or were treated with PBS followed by immunization @`�HW0Y_�:
with OVA(323–339) (primed) or with CTLA-4–Ig plus mAb to CD40L followed by K�D�'}9{F,
immunization with OVA(323–339) as described above (tolerized). Then, 3 d later, ;kD
�R�m'(
lymphocytes were isolated from the draining lymph nodes of the BALB/c hosts. The Nb\B*=4�AR
number of cell divisions on CFSE-stained cells and the percentage of cells that had f5�'vjWJ30
undergone a specific number of divisions were determined as described43. Cells were also +<WNAmh
��
stained with mAb KJ1-26 and CFSE analysis of KJ1-26+ T cells was done by flow `(~oZbE�rM
cytometry. cq8JpS�B�(
Adenovirus vectors. Jv~^�hN�2�
The cDNA encoding Ras61L was provided by F. Fitch (University of Chicago, Chicago, ��]F"@+_E�
Illinois). The dominant negative Cbl construct was generated by RT-PCR with cDNA xxpzz(S ]A
from TH1 clones as a template and the following primers (upper case, restriction enzyme m��A5sK?W�
sequences; underlining, Myc tag sequence): �"f-HOd\=�
5'-GGGGTACCatggagcagaaactcatctctgaagaggatctggccggcaacgtgaagaaga-3' (forward) and �{ApjOIxk�
5'-ATAGTTTAGCGGCCGCtcaatcttgaggagttggtt cacataa-3' (reverse). The cDNA �g�V�s@T'�
encoding DGK- was a gift from M. Topham (University of Utah, Salt Lake City, Utah) Q� 2����B�
and was used as a template to introduce an N-terminal Myc epitope tag by PCR. The #m3!U�(Og`
sequences of all PCR products were confirmed before subcloning. Construction of ]x6�r��
P�
recombinant adenovirus vectors was done with a two-cosmid system that has been �����iT<�/
described42. LPkl16��yZ
Adenoviral transduction of CAR T cells. � �B�m&�6
TH1 clones were purified from passage cultures by Ficoll-Hypaque centrifugation. `?S�L��p��
Primary CAR 2C Rag2-/- CD8+ T cells were isolated from splenocytes by negative &,$N|$yK}|
selection with magnetic beads and antibody 'cocktails' (Stem Cell Technologies). CAR <BK�?�@X�y
TH1 cells were transduced with adenovirus vectors at high cell density (1 107 cells/ml) e�q
qnR�.0
in DMEM containing 2% (volume/volume) FCS and were incubated for 1 h at 37 °C, S�4
s#ED�s
16 |�q
Pu*�vR
followed by an overnight 'rest' at 37 °C in DMEM containing 5% (volume/volume) FCS "1rT>
ASWI
at low cell density (4 105 cells/ml). BVS�
SO's�
Lentivirus production and infection protocols. �9y�j'->dL
A third-generation lentiviral vector encoding EGFP expressed from the human ]�a�YuB�oj
phosphoglycerate kinase promoter was used as described29, 33. Cell populations were �YAd�%d
|Q
incubated overnight (about 16 h) in X-VIVO-10 medium (BioWhittaker) supplemented rW�`l1yi*$
with 1% BSA (Stem Cell Technologies) and L-glutamine (Invitrogen) with viral ~Sx\>w�Blc
supernatant (multiplicity of infection of 130–180). Viral concentrations of 1.0 108 to 1.8 6u{%jSA>D\
108 viral particles/ml, 2.0 107 to 4.4 107 viral particles/ml and 0.9 108 to 1.6 108 3]k�N�9n�{
viral particles/ml and cell concentrations of 0.7 106 to 1.1 106 cells/ml, 1.0 105 to 2.5 Fm+V_.H/;�
105 cells/ml and 0.7 106 to 1.4 106 cells/ml for CD34+CD38lo, CD34+CD38- and Lin- #j"GS�/y"�
cord blood, respectively, were maintained. The efficiency of gene transfer was estimated SA�?1*dw�)
by progenitor cell assay as described33. �r"dR}S.Uf
Apoptosis induction. Y ��/l�~R7
Spontaneous apoptosis of PMNs was detected after 22 h of incubation in culture media. 9�rT"�_d�#
In some experiments, zVAD-fmk (10-50 M), TNF (40 ng/ml), resolvin E1–methyl ester, \���!IE��Z
aspirin-triggered lipoxin A4 analog, PD1–methyl ester (10 nM) or TGF- (10 ng/ml) was �lz�_��� r
added. Vehicle treatment was 0.05% (volume/volume) ethanol. Peripheral blood T cells xsU3c0wbr8
were activated by incubation for 3 d in 24-well plates coated with anti-CD3 (5 g/ml; kR�{$&�cE^
R&D Systems). Jurkat cells or activated peripheral blood T cells were incubated for 4–48 �uF�FC.��w
h with staurosporine (1–2 M) or Fas ligand (0.05–5 ng/ml), after which cells were c�hM�-YuN|
collected and used for flow cytometry or binding assays. In some experiments, �o ��Va�[�
zVAD-fmk (10–50 M; R&D Systems) was added to cells 20 min before the addition of :bX�TV?#0
apoptosis-indu X�Y�<KLO�%
Mice strains and genotyping. 3V<c4'O\W�
The 129/Sv Rhoh-/- mice were generated by Targeting Laboratory. The entire coding V�O�T9cP^6
region of mouse Rhoh is in its third exon; the targeting vector was designed to replace the n��PH\Lra�
third exon of Rhoh with a neomycin-resistance cassette. The genotypes of Rhoh !�(y(6�u#
gene-targeted embryonic stem cells and transgenic mice were determined by Southern ��SBY0
L.�
blot analysis of DNA digested with SpeI using a 5' Rhoh genomic DNA probe or by PCR 9���7pnq1b
analysis with primers. The 129/Sv Rhoh-/- mice were crossed with wild-type or p14 TCR zbfe=J4��c
(V 2V 8) transgenic mice on a C57BL/6J background to generate Rhoh-/- or (��Z8wMy&:
p14tg/+Rhoh-/- compound mice. Mice used were littermates derived from backcross ?�<^^.��Si
generations with an N of more than 2. The 129S6/SvEvTac-Rag2-/- mice were purchased qJ�R8fQ���
from Taconic Animal Models. All animal experiments were approved by the Institutional EF;B)���y=
Animal Care and Use Committee of the Cincinnati Children's Hospital Research �&"Fz���)}
Foundation (Cincinnati, Ohio). ,2�P��/[ :
Antibodies and GST fusion proteins. m;�PTO�$--
17 1+V�e�i<H$
Fluorescence-conjugated monoclonal antibodies to the following mouse antigens were ��#r�]GnC,
used for flow cytometry: CD4 (RM4-5), CD8 (53-6.7), CD25 (7D4), CD44 (IM7), TCR .:tR*Kst`7
-chain (H57-597), TCR (GL3), TCR V 8, TCR V 5 (MR9-4), CD69 (H1.2F3), CD5 wkT4R\H�>�
(53-7.3), Gr-1 (RB6-8C5), Mac-1 (M1-70), NK1.1 (PK136), Thy1.2 (53-2.1), �� nWUau:%
CD45R–B220 (RA3-6B2), IgM (R6-60.2), BrdU (3D4) and Ter119 (Ly-76; all from P#"_H�}qC*
Pharmingen). For immunoblot analyses, antibodies to the following were used: RhoH9 ,QLy��}=N�
(B4998), Zap70 phosphorylated at Y319 (17a), phosphorylated tyrosine (4G10) and Lat o_���r{cnu
(45; Pharmingen); hemagglutinin (3F10; Roche); -actin (AC-15; Sigma); CD3 5xa!L@)`wF
(6B10.2; Santa Cruz Biotechnology); and Lat phosphorylated at Y191 (3584), Zap70 ��@��9\��E
(99F2), phosphorylated p42-p44 (Thr202-Tyr204; 197G2) and p42-p44 (9102; Cell xFyBF�[c��
Signaling Technology). Primary antibodies were detected with the secondary antibodies 4ZB]n,�pfT
horseradish peroxidase–conjugated goat anti-mouse (7076) or goat anti-rabbit (7074; both >uE<-klv��
Cell Signaling Technology), or donkey anti-rat (sc-2956; Santa Cruz Biotechnology) G��z7,�g
Y
using enhanced chemiluminescence detection (Cell Signaling Technology). GST fusion Zm#,I�ke?#
proteins were expressed in Escherichia coli BL21 (DE3) cells and were purified <XzRRC�YQ�
according to the manufacturer's recommendations (GE Healthcare Life Science). Purified M*�dou_��Q
GST fusion protein lysates were incubated for 1 h at 4 °C with glutathione–Sepharose 4B D?"Q)kV�uD
beads. Bead-bound GST fusion proteins were separated by SDS-PAGE and were T? ,���Q=.
quantified by Coomassie blue staining. ��6>h"Lsww
GST precipitation assay. kZ!&3G9�>-
Jurkat cells were lysed in GST lysis buffer (50 mM Tris-HCl, pH 7.5, 150 mM NaCl, 10 (�
R!.=95@
mM MgCl2, 1% Nonidet-P40 and Complete Protease Inhibitors). Cell lysates were loaded cN�)no�Gkp
onto columns of bead-bound GST fusion proteins. After columns were washed with GST &�CfzhIi*!
lysis buffer containing 150 mM and 200 mM NaCl, bound proteins were eluted with GST �tz2$j
@!=
lysis buffer containing 400 mM NaCl and SDS sample buffer, sequentially. Eluted �`�U�{#;��
proteins were detected by SDS-PAGE and Coomassie blue staining. Protein bands were y�Rz� l}��
identified with a Bruker Biflex III MALDI-TOF mass spectrometer (SpectroREADER; �DhG{h�Q[[
Sequenom) and Protein Mass Fingerprinting Mascot search (Matrix Science). B:)vPO�+ d
Subcellular fractionation. RR>G}u9�np
Cells were lysed by brief sonication on ice in a buffer of 250 mM sucrose, 20 mM Tris, �^!S�wY�_>
pH 7.8, 10 mM MgCl2, 1 mM EDTA, 1 mM Na3VO4, 10 mM NaF and Complete oSP^
.�BJ$
Protease Inhibitors. Lysates were centrifuged to remove nuclei and debris (900g for 5 min �mm N��$\2
at 4 °C). The P100 and S100 fractions were separated by centrifugation for 30 min at W}�k)5<C4v
100,000g. Membrane fractions were made soluble with MLB (Upstate) plus protease and �'he&�h4fm
phosphatase inhibitors. After centrifugation for additional 30 min at 100,000g, the �?)4c�!3#�
detergent-insoluble cytoskeleton-containing fraction was resolved by 0.5% SDS-PAGE. �/-g%�IeF
Assessment of Intracellular Calcium Concentration {;�hR�FQ^b
