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HEMATOPOIESIS
From the Office of Clinical Research and Laboratory of
Signal Transduction, National Institute of Environmental Health
Sciences, Research Triangle Park, NC; and Departments of Medicine and
Biochemistry, Duke University Medical Center, Durham, NC.
Tristetraprolin (TTP) is a member of the CCCH tandem zinc-finger
class of proteins. It can bind to and destabilize mRNAs encoding tumor necrosis factor- Tristetraprolin (TTP), also known as TIS11, Nup475,
or G0S24,1-4 is the prototype of a recently described
family of zinc-finger proteins of the CCCH class.5 Mice
deficient in TTP develop a severe syndrome characterized by growth
retardation and cachexia, polyarticular arthritis, dermatitis,
autoimmunity, and myeloid hyperplasia accompanied by extramedullary
hematopoiesis.6 The involvement of tumor necrosis
factor- Further studies using macrophages derived from either fetal liver or
bone marrow showed increased production of TNF- A second aspect of the phenotype was revealed when we found that bone
marrow stromal cells (BMSCs) derived from TTP-deficient mice exhibited
increased production of the hematopoietic growth factor and
proinflammatory cytokine granulocyte-macrophage colony-stimulating factor (GM-CSF).13 As in the case of TNF- TNF- In an attempt to determine which aspects of the TTP-associated
phenotype are mediated by each receptor, we generated mice deficient in
both TNFRs and TTP, and also animals that were deficient in TTP and
each individual receptor. We show here that TNFR1 is responsible for
the development of arthritis and cachexia in the absence of TTP. These
studies confirm the involvement of TNF- Mice
Histology
Cell culture Bone marrow-derived macrophages (BMM s) were prepared as
described previously.10 Briefly, marrow cells were flushed
from both femurs of individual mice and cultured at 37°C in a 5%
CO2 atmosphere. The culture medium was Eagle's modified
minimum essential medium, supplemented with 10% (vol/vol)
heat-inactivated fetal calf serum, 2 mM glutamine, 100 U/mL penicillin,
100 µg/mL streptomycin, 1.25 µg/mL amphotericin B, 0.2% sodium
bicarbonate, 15 mM HEPES, pH 7.4, and 30% (vol/vol) L929
cell-conditioned medium as a source of macrophage colony-stimulating
factor.27 Cells were used after 2 to 3 weeks in culture.
BMSCs were prepared as described previously.13 Briefly,
marrow cells were flushed from both femurs of individual mice, and red
blood cells were lysed with 0.15 M ammonium chloride. Cells were
cultured at 33°C in a 5% CO2 atmosphere in minimum
essential medium- Northern blotting To study the induction of TTP gene expression by TNF- , we
incubated BMMs with increasing doses of recombinant mouse TNF- (rmTNF-, 0-10 ng/mL; R&D Systems, Minneapolis, MN) for 30 minutes. RNA was extracted using the RNeasy kit from Qiagen (Valencia, CA)
according to the directions of the manufacturer. RNA was analyzed by
Northern blot on 1.5% (wt/vol) agarose gels, and blots were hybridized with a mouse TTP cDNA.3
Similarly, induction of GM-CSF and TNF- GM-CSF and TNF-
Phenotypes of the TTP/TNFR-deficient mice Development. Mice deficient in TNFR1, TNFR2, or both have been described previously,20,22 and all of them appear to develop normally. Their weights are comparable to those of wild-type (WT) mice, and they do not show any obvious signs of disease. We generated mice that were deficient in TTP and both TNFRs (3KO) and also mice deficient in TTP and each individual receptor (TTP/TNFR1KO or TTP/TNFR2KO). The TTPKO mice used in this study had been back-crossed into C57Bl/6 mice for an average of 11 generations (range, 10-12 generations). Controls were mice deficient in either or both TNFRs. At 5 weeks of age, growth retardation was already apparent in the TTPKO mice (average body weight, 7.8 ± 2.1 g, n = 4, versus 18.1 ± 1.4 g in the WT mice, n = 7) (mean ± SD) (P < .0001). Mice of the 3KO and the TTP/TNFR1KO genotypes exhibited the same rate of growth as the WT animals (18.3 ± 2.2 g, n = 16, and 18.1 ± 1.7 g, n = 14, respectively). On the other hand, the average weight of the TTP/TNFR2KO mice at 5 weeks was 9 ± 2.7 g (n = 5) (P < .03 compared with WT). After 12 weeks, the pattern remained the same: WT, 23.7 ± 2.2 g (n = 7); TTPKO, 9.3 ± 2.1 g (n = 4); 3KO, 23.7 ± 2.2 g (n = 16); TTP/TNFR1KO, 23.8 ± 3.1 g (n = 14); and TTP/TNFR2KO, 12.4 ± 0.5 g (n = 5). However, at 20 weeks of age, mice of the 3KO and TTP/TNFR1KO genotypes appeared to slow in their weight gain: WT, 33.1 ± 0.1 g (n = 4); 3KO, 25.2 ± 2.9 g (n = 16); and TTP/TNFR1KO, 26.3 ± 4 g (n = 14). At 5 weeks of age, there were no obvious physical abnormalities in the 3KO or TTP/TNFR1KO mice. However, by this age the TTP/TNFR2KO mice already displayed early signs of joint inflammation, characterized by swelling and discoloration of the paws (Figure 1). This onset of inflammation occurred earlier than in the TTPKO mice, which did not show signs of paw joint inflammation until 8 to 10 weeks of age. These paw changes were not seen in the other genotypes, even after several months of observation (data not shown). Over time, the TTP/TNFR2 mice rapidly deteriorated, as did the TTPKO mice, whereas the TTP/TNFR1KO and 3KO mice continued to develop normally and without signs of disease (except for the leveling off of the weight gain that occurs after 5 months of age). Both of these genotypes were fertile and able to carry gestation to term, and both had normal litter sizes and reared the pups normally. Breeding was not attempted with the homozygous TTP/TNFR2KO mice.
Histology.
Carpal joints of adult mice were examined histologically at
approximately 6 months of age (Figure 2).
The 3KO (Figure 2A) and the TTP/TNFR1KO mice (Figure 2B) exhibited no
signs of joint inflammation, in agreement with the external examination
of the animals. However, in the TTP/TNFR2KO mice (Figure 2C), the
histology of the joint was markedly abnormal, with severe erosion of
the articular surfaces, invasion of the joint cavities by inflammatory pannus, and dramatic infiltration of the surrounding soft tissues by
mononuclear and polymorphonuclear inflammatory cells (Figure 2D). This
pathology was very similar to that described in the TTPKO
mice,6 but appeared to be more aggressive in both extent and earlier age at onset.
Microscopic examination of the bone marrow cavities from mice of all 3 TTP-deficient genotypes (Figure 2) revealed the hypercellular marrow that is typical of the TTPKO mice.6 In the present study, this marrow hypercellularity was present even in the absence of both TNFRs. Cell preparations of bone marrow from animals expressing TTP (Figure 3, panels WT and TNFR1/2KO) showed a heterogeneous population of cells, including members of the 3 hematopoietic lineages (lymphoid, myeloid, and erythroid). In contrast, whenever TTP was absent (Figure 3, panels TTPKO, 3KO, TTP/TNFR1KO, and TTP/TNFR2KO), there was a marked increase in the proportion of myeloid cells at all stages of differentiation, with almost complete disappearance of the lymphoid and erythroid lineages. The percentages of myeloid cells in these genotypes were as follows: TTPKO, 77% ± 2.1% (n = 3); 3KO, 68.3% ± 2.6% (n = 6); TTP/TNFR1KO, 64.7% ± 4% (n = 3); and TTP/TNFR2KO, 72.2% ± 5% (n = 4) (mean ± SEM). In each case, this represents at least a 2-fold increase in the proportion of myeloid cells compared with marrow from WT mice (30.4% ± 3% [n = 7]).
These results were somewhat unexpected because TTP-deficient mice treated with neutralizing antibodies to TNF- for 8 weeks did not
exhibit significant myeloid hyperplasia at 73 days of age compared with
control animals (33.7% ± 3.1% marrow myeloid cells in the
antibody-treated KO mice versus 30.4% ± 3.0% in control mice).6 Because these mice were considerably younger than
the 3KO mice evaluated in the present study, we analyzed marrow from 3KO mice at 82 days of age. Marrow from these mice contained
37.5% ± 2.5% myeloid cells (n = 4), suggesting strongly that the
severe myeloid hyperplasia seen in the older 3KO mice was an
age-related effect of the abnormal genotype that was not apparent
either in the younger mice treated with TNF- antibodies or in the
younger 3KO mice.
In the TTPKO mouse, myeloid hyperplasia in the bone marrow is always
accompanied by extramedullary hematopoiesis, particularly in the
spleen, which is almost always significantly enlarged.6 This phenomenon was also seen in the 3KO and TTP/TNFR1KO mice older
than 6 months of age; the spleens of these animals weighed up to 700 mg
(normal, less than 100 mg). Even when splenomegaly was not as obvious,
the normal architecture of the spleen was altered in the 3 genotypes
lacking TTP. Spleens from TNFR1/2KO mice (Figure
4) appeared in all respects to be similar
to those of the WT mice (not shown), with normal architecture of the
white and red pulps and a population of predominantly lymphoid cells, with the occasional mature granulocyte. However, spleens from animals
of the other 3 genotypes, in which TTP was absent, were strikingly
similar to the spleens of the TTPKO mice,6 with increased
numbers of myeloid precursors at different stages of differentiation
(Figure 4, panels 3KO, TTP/TNFR1KO, and TTP/TNFR2KO). In addition,
increased numbers of megakaryocytes were observed, as in the original
TTPKO mice (E.C. and P.J.B., unpublished observations, 1998-2001).
Involvement of TNFR1 and TNFR2 in the expression of TTP To evaluate the role played by each TNFR in the induction of TTP expression by TNF-, we incubated BMMs for 30 minutes in the
presence of increasing concentrations of rmTNF-, and then isolated
and analyzed RNA by Northern blot. In WT BMMs, TTP mRNA accumulation
was first detected after exposure to 0.1 ng/mL rmTNF- for 30 minutes
(Figure 5). In the absence of both TNFR1
and TNFR2, TNF- caused no increase in TTP mRNA accumulation. The
absence of TNFR1 alone also completely prevented rmTNF--induced TTP
mRNA accumulation. When TNFR1 alone was present, rmTNF- induced TTP mRNA accumulation. However, there was a clear shift to the right in the
rmTNF- concentration needed to trigger this response. In the cells
of this genotype, no increase in TTP mRNA accumulation was seen after
exposure to 0.1 ng/mL rmTNF-, and even 10 ng/mL rmTNF- stimulated
less TTP mRNA accumulation than that seen in the cells from the
WT animals.
Involvement of TNFR1 and TNFR2 in the expression and stability of GM-CSF mRNA We also examined the role played by each TNFR in the induction of GM-CSF mRNA. In WT BMSCs, GM-CSF mRNA was detected after 2 hours of exposure to 0.1 ng/mL rmTNF- (Figure
6). The absence of TNFR1 resulted in the
complete lack of expression of GM-CSF mRNA, even after the highest dose
of rmTNF- was used (10 ng/mL). However, although in the absence of
TNFR2 there was TNF- induction of GM-CSF mRNA accumulation, there
was a shift to the right in the concentration of rmTNF- required for
the first detectable expression of GM-CSF mRNA. In the absence of
TNFR2, GM-CSF mRNA was first detected only after a 2-hour incubation in
the presence of 1 ng/mL rmTNF-, in contrast to 0.1 ng/mL in the
WT cells.
We also evaluated which TNFR was involved in the regulation of GM-CSF
mRNA stability. To do this, we compared the half-life of GM-CSF mRNA
after actinomycin D treatment of BMSCs stimulated for 2 hours with 1 µg/mL LPS. In the TNFR1KO and TNFR2KO cells, the larger
(polyadenylated) form of GM-CSF mRNA decayed very quickly after
actinomycin D treatment, whereas the smaller (deadenylated) form13 decreased with a somewhat longer half-life (Figure
7). The estimated half-life of both mRNA
species combined was 35 minutes and 39 minutes for the 2 genotypes,
respectively. However, when the BMSCs were derived from the TTP/TNFR1KO
cells, the decay of the polyadenylated form of the mRNA was somewhat
delayed, with an estimated half-life of 49 minutes. In the absence of
both TTP and TNFR2, there was little detectable deadenylated GM-CSF
mRNA, and the half-life of the total mRNA was greatly increased (415 minutes).
Involvement of TNFR1 and TNFR2 in the expression and stability of
TNF- mRNA. TNFR2 alone failed to mediate the rmTNF--mediated expression of TNF- in BMSCs (Figure
8). In contrast, TNFR1 was able to
mediate the rmTNF--stimulated expression of TNF-, but higher
concentrations of rmTNF- were required to achieve the same response
as that seen in the WT cells. Accumulation of TNF- mRNA was readily
detectable after exposure of the WT BMSCs to 0.01 ng/mL rmTNF-,
whereas it was not detectable until a concentration of 0.1 ng/mL was
used in the TNFR2KO BMSCs.
Finally, because TNF-
The main goal of the present study was to establish the role
played by TNF- A second goal of these studies was to explore the involvement of each
TNFR in the development of the TTP-deficiency phenotype. Previous
studies have demonstrated that each TNFR appears to be responsible for
certain, sometimes overlapping actions of TNF- The results presented here demonstrate that TNFR1 and TNFR2 play distinct roles in the development of the TTP deficiency-associated phenotype. The superimposition of TNFR1 deficiency on TTP deficiency resulted in prevention of the cachexia and arthritis characteristic of this syndrome, resulting in a phenotype that was very similar to that exhibited by the 3KO mice. The TTP/TNFR1KO mice, like the 3KO mice, developed normally and bred well, and we were able to produce a colony of homozygous mice. However, as seen in the 3KO mice, as the mice aged past approximately 6 months, they began to develop myeloid hyperplasia and extramedullary hematopoiesis with splenomegaly, and their growth rates dropped below those of control mice. In contrast, the combined deficiency of TTP and TNFR2 resulted in a
very different phenotype. These mice appeared similar to the TTPKO
mice, with cachexia and growth impairment obvious at an early age.
These animals also developed severe polyarticular arthritis of the paw
joints, but the onset appeared to be earlier than in the TTPKO mice.
TTPKO mice generally exhibit signs of discoloration and swelling in the
paw joints at 8 to 10 weeks of age, but these signs were
apparent as early as 3 to 4 weeks of age in the TTP/TNFR2KO
mice. Histology of the paw joints confirmed the very early onset of
erosive arthritis. As with all of the other genotypes lacking TTP, the
TTP/TNFR2KO mice also developed myeloid hyperplasia and extramedullary
hematopoiesis as they aged. Both the TTPKO and TTP/TNFR2KO mice were
produced by crossing heterozygotes because both homozygous lines have
very low breeding capabilities. In both cases, regardless of the
severity of the postnatal syndrome, both TTPKO and TTP/TNFR2KO mice
were born at the appropriate mendelian rates, suggesting that the
excess TNF- Two main conclusions can be drawn from these data. First, TNF- All of the animals studied that were deficient in TTP displayed myeloid
hyperplasia and extramedullary hematopoiesis after about 6 to 8 months
of age, including those also deficient in one or both TNFRs. This
appears to be an age-related phenomenon because the 3KO animals did not
exhibit myeloid hyperplasia when examined at 82 days of age, in keeping
with our previous results with the TNF- We have previously suggested a model in which TTP regulates TNF- Finally, our results suggest an involvement of TNFR1 in the
TNF- In conclusion, using the inflammatory disease model provided by the
TTPKO mice, we have been able to differentiate the roles played by each
TNFR in the regulation of key components of the inflammatory response,
including TNF-
We thank Drs J. Bonner and D. Germolec for critical reading of
the manuscript and Dr W. S. Lai for the TNF-
Submitted April 18, 2001; accepted June 15, 2001.
The publication costs of this article were defrayed in part by page charge payment. Therefore, and solely to indicate this fact, this article is hereby marked "advertisement" in accordance with 18 U.S.C. section 1734.
Reprints: Perry J. Blackshear, National Institute of Environmental Health Sciences, MD A2-05, PO Box 12233, Research Triangle Park, NC 27709; e-mail: black009{at}niehs.nih.gov.
1.
DuBois RN, McLane MW, Ryder K, Lau LF, Nathans D.
A growth factor-inducible nuclear protein with a novel cysteine/histidine repetitive sequence.
J Biol Chem.
1990;265:19185-19191 2. Heximer SP, Forsdyke DR. A human putative lymphocyte G0/G1 switch gene homologous to a rodent gene encoding a zinc-binding potential transcription factor. DNA Cell Biol. 1993;12:73-88[Medline] [Order article via Infotrieve].
3.
Lai WS, Stumpo DJ, Blackshear PJ.
Rapid insulin-stimulated accumulation of an mRNA encoding a proline-rich protein.
J Biol Chem.
1990;265:16556-16563 4. Varnum BC, Lim RW, Sukhatme VP, Herschman HR. Nucleotide sequence of a cDNA encoding TIS11, a message induced in Swiss 3T3 cells by the tumor promoter tetradecanoyl phorbol acetate. Oncogene. 1989;4:119-120[Medline] [Order article via Infotrieve].
5.
Varnum BC, Ma QF, Chi TH, Fletcher B, Herschman HR.
The TIS11 primary response gene is a member of a gene family that encodes proteins with a highly conserved sequence containing an unusual Cys-His repeat.
Mol Cell Biol.
1991;11:1754-1758 6. Taylor GA, Carballo E, Lee DM, et al. A pathogenetic role for TNF alpha in the syndrome of cachexia, arthritis, and autoimmunity resulting from tristetraprolin (TTP) deficiency. Immunity. 1996;4:445-454[CrossRef][Medline] [Order article via Infotrieve].
7.
Cheng J, Turksen K, Yu QC, Schreiber H, Teng M, Fuchs E.
Cachexia and graft-vs.-host-disease-type skin changes in keratin promoter-driven TNF alpha transgenic mice.
Genes Dev.
1992;6:1444-1456 8. Keffer J, Probert L, Cazlaris H, et al. Transgenic mice expressing human tumour necrosis factor: a predictive genetic model of arthritis. EMBO J. 1991;10:4025-4031[Medline] [Order article via Infotrieve]. 9. Ulich TR, Shin SS, del Castillo J. Haematologic effects of TNF. Res Immunol. 1993;144:347-354[CrossRef][Medline] [Order article via Infotrieve].
10.
Carballo E, Gilkeson GS, Blackshear PJ.
Bone marrow transplantation reproduces the tristetraprolin-deficiency syndrome in recombination activating gene-2 (
11.
Carballo E, Lai WS, Blackshear PJ.
Feedback inhibition of macrophage tumor necrosis factor-alpha production by tristetraprolin.
Science.
1998;281:1001-1005
12.
Lai WS, Carballo E, Strum JR, Kennington EA, Phillips RS, Blackshear PJ.
Evidence that tristetraprolin binds to AU-rich elements and promotes the deadenylation and destabilization of tumor necrosis factor alpha mRNA.
Mol Cell Biol.
1999;19:4311-4323
13.
Carballo E, Lai WS, Blackshear PJ.
Evidence that tristetraprolin is a physiological regulator of granulocyte-macrophage colony-stimulating factor messenger RNA deadenylation and stability.
Blood.
2000;95:1891-1899
14.
Koeffler HP, Gasson J, Tobler A.
Transcriptional and posttranscriptional modulation of myeloid colony-stimulating factor expression by tumor necrosis factor and other agents.
Mol Cell Biol.
1988;8:3432-3438 15. Hill CM, Lunec J. The TNF-ligand and receptor superfamilies: controllers of immunity and the Trojan horses of autoimmune disease? Mol Aspects Med. 1996;17:455-509[CrossRef][Medline] [Order article via Infotrieve].
16.
Pinckard JK, Sheehan KC, Schreiber RD.
Ligand-induced formation of p55 and p75 tumor necrosis factor receptor heterocomplexes on intact cells.
J Biol Chem.
1997;272:10784-10789 17. Barbara JA, Smith WB, Gamble JR, et al. Dissociation of TNF-alpha cytotoxic and proinflammatory activities by p55 receptor- and p75 receptor-selective TNF-alpha mutants. EMBO J. 1994;13:843-850[Medline] [Order article via Infotrieve]. 18. Mukherjee R, Singh S, Chaturvedi MM, Aggarwal BB. Evidence for a synergistic role of two types of human tumor necrosis factor receptors for the ligand-dependent activation of the nuclear transcription factor NF-kappaB. J Interferon Cytokine Res. 1998;18:117-123[Medline] [Order article via Infotrieve]. 19. Pfeffer K, Matsuyama T, Kundig TM, et al. Mice deficient for the 55 kd tumor necrosis factor receptor are resistant to endotoxic shock, yet succumb to L. monocytogenes infection. Cell. 1993;73:457-467[CrossRef][Medline] [Order article via Infotrieve]. 20. Rothe J, Lesslauer W, Lotscher H, et al. Mice lacking the tumour necrosis factor receptor 1 are resistant to TNF-mediated toxicity but highly susceptible to infection by Listeria monocytogenes. Nature. 1993;364:798-802[CrossRef][Medline] [Order article via Infotrieve].
21.
Bigda J, Beletsky I, Brakebusch C, et al.
Dual role of the p75 tumor necrosis factor (TNF) receptor in TNF cytotoxicity.
J Exp Med.
1994;180:445-460 22. Erickson SL, de Sauvage FJ, Kikly K, et al. Decreased sensitivity to tumour-necrosis factor but normal T-cell development in TNF receptor-2-deficient mice. Nature. 1994;372:560-563[CrossRef][Medline] [Order article via Infotrieve]. 23. Grell M, Douni E, Wajant H, et al. The transmembrane form of tumor necrosis factor is the prime activating ligand of the 80 kDa tumor necrosis factor receptor. Cell. 1995;83:793-802[CrossRef][Medline] [Order article via Infotrieve].
24.
Jacobsen FW, Rothe M, Rusten L, et al.
Role of the 75-kDa tumor necrosis factor receptor: inhibition of early hematopoiesis.
Proc Natl Acad Sci U S A.
1994;91:10695-10699
25.
Tartaglia LA, Pennica D, Goeddel DV.
Ligand passing: the 75-kDa tumor necrosis factor (TNF) receptor recruits TNF for signaling by the 55-kDa TNF receptor.
J Biol Chem.
1993;268:18542-18548 26. Weiss T, Grell M, Hessabi B, et al. Enhancement of TNF receptor p60-mediated cytotoxicity by TNF receptor p80: requirement of the TNF receptor-associated factor-2 binding site. J Immunol. 1997;158:2398-2404[Abstract]. 27. Hume DA, Gordon S. Optimal conditions for proliferation of bone marrow-derived mouse macrophages in culture: the roles of CSF-1, serum, Ca2+, and adherence. J Cell Physiol. 1983;117:189-194[CrossRef][Medline] [Order article via Infotrieve]. 28. Sheehan KC, Ruddle NH, Schreiber RD. Generation and characterization of hamster monoclonal antibodies that neutralize murine tumor necrosis factors. J Immunol. 1989;142:3884-3893[Abstract].
29.
Metcalf D, Elliott MJ, Nicola NA.
The excess numbers of peritoneal macrophages in granulocyte-macrophage colony-stimulating factor transgenic mice are generated by local proliferation.
J Exp Med.
1992;175:877-884 30. Mohler KM, Torrance DS, Smith CA, et al. Soluble tumor necrosis factor (TNF) receptors are effective therapeutic agents in lethal endotoxemia and function simultaneously as both TNF carriers and TNF antagonists. J Immunol. 1993;151:1548-1561[Abstract]. 31. Wooley PH, Dutcher J, Widmer MB, Gillis S. Influence of a recombinant human soluble tumor necrosis factor receptor FC fusion protein on type II collagen-induced arthritis in mice. J Immunol. 1993;151:6602-6607[Abstract].
© 2001 by The American Society of Hematology.
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  D. J. Stumpo, H. E. Broxmeyer, T. Ward, S. Cooper, G. Hangoc, Y. J. Chung, W. C. Shelley, E. K. Richfield, M. K. Ray, M. C. Yoder, et al. Targeted disruption of Zfp36l2, encoding a CCCH tandem zinc finger RNA-binding protein, results in defective hematopoiesis Blood, September 17, 2009; 114(12): 2401 - 2410. [Abstract] [Full Text] [PDF]
|
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|
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 |
|
 A. M. S. Hartz, B. Bauer, M. L. Block, J.-S. Hong, and D. S. Miller Diesel exhaust particles induce oxidative stress, proinflammatory signaling, and P-glycoprotein up-regulation at the blood-brain barrier FASEB J, August 1, 2008; 22(8): 2723 - 2733. [Abstract] [Full Text] [PDF]
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 |
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 W. S. Lai, J. S. Parker, S. F. Grissom, D. J. Stumpo, and P. J. Blackshear Novel mRNA Targets for Tristetraprolin (TTP) Identified by Global Analysis of Stabilized Transcripts in TTP-Deficient Fibroblasts Mol. Cell. Biol., December 15, 2006; 26(24): 9196 - 9208. [Abstract] [Full Text] [PDF]
|
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D. J. Stumpo, N. A. Byrd, R. S. Phillips, S. Ghosh, R. R. Maronpot, T. Castranio, E. N. Meyers, Y. Mishina, and P. J. Blackshear Chorioallantoic Fusion Defects and Embryonic Lethality Resulting from Disruption of Zfp36L1, a Gene Encoding a CCCH Tandem Zinc Finger Protein of the Tristetraprolin Family Mol. Cell. Biol., July 15, 2004; 24(14): 6445 - 6455. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 P. Anderson, K. Phillips, G. Stoecklin, and N. Kedersha Post-transcriptional regulation of proinflammatory proteins J. Leukoc. Biol., July 1, 2004; 76(1): 42 - 47. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 H. Cao, J. S. Tuttle, and P. J. Blackshear Immunological Characterization of Tristetraprolin as a Low Abundance, Inducible, Stable Cytosolic Protein J. Biol. Chem., May 14, 2004; 279(20): 21489 - 21499. [Abstract] [Full Text] [PDF]
|
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|
|
 |
|
 K. Phillips, N. Kedersha, L. Shen, P. J. Blackshear, and P. Anderson Arthritis suppressor genes TIA-1 and TTP dampen the expression of tumor necrosis factor {alpha}, cyclooxygenase 2, and inflammatory arthritis PNAS, February 17, 2004; 101(7): 2011 - 2016. [Abstract] [Full Text] [PDF]
|
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 |
|
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|
|
|
|
|
|
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|
|
|
|
|
|
B. A. Johnson, J. R. Stehn, M. B. Yaffe, and T. K. Blackwell Cytoplasmic Localization of Tristetraprolin Involves 14-3-3-dependent and -independent Mechanisms J. Biol. Chem., May 10, 2002; 277(20): 18029 - 18036. [Abstract] [Full Text] [PDF]
|
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W. S. Lai, E. A. Kennington, and P. J. Blackshear Interactions of CCCH Zinc Finger Proteins with mRNA. NON-BINDING TRISTETRAPROLIN MUTANTS EXERT AN INHIBITORY EFFECT ON DEGRADATION OF AU-RICH ELEMENT-CONTAINING mRNAs J. Biol. Chem., March 8, 2002; 277(11): 9606 - 9613. [Abstract] [Full Text] [PDF]
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receptor subtypes in the
pathogenesis of the tristetraprolin-deficiency syndrome
Top
Abstract
Introduction
/