蛋白质磷酸化调控羊肉肌原纤维蛋白的功能

【目的】通过激活蛋白激酶的活性提高羊肉肌原纤维蛋白的磷酸化水平,分析磷酸化水平的提高对羊肉肌原纤维蛋白降解程度、收缩功能的影响,进一步揭示蛋白质磷酸化对羊肉肌肉嫩化的作用机理。【方法】通过添加蛋白激酶A激活剂Forskolin、蛋白激酶C激活剂佛波酯（PMA）,提高蛋白激酶的活性,改变羊肉肌原纤维蛋白的磷酸化水平。比较激活剂处理组与空白对照组肌原纤维小片化指数（MFI）、条带降解程度、肌节长度等指标的差异,确定蛋白质磷酸化水平对羊肉肌肉收缩和肌肉降解的影响。【结果】将羊肉样品在蛋白激酶溶液中培养24 h,在培养结束后1、2和4 h,PMA处理组（PKC激活组）的蛋白激酶活性显著高于空白对照组（P＜0.05）,而在培养后1和4 h,Forskolin处理组（PKA激活组）的蛋白激酶活性显著高于空白对照组（P＜0.05）。PMA处理组和Forskolin处理组的最高蛋白激酶活性出现在培养后1 h。Forskolin和PMA通过提高激酶活性显著提高肌联蛋白（Titin）、肌球蛋白结合蛋白C（Myosin binding protein C）、原肌球蛋白（Tropomyosin）、肌球蛋白轻链2（Myosin light chain 2）等蛋白质的磷酸化水平,肌球蛋白重链、肌动蛋白质的磷酸化水平没有显著变化,Forskolin组和PMA组的蛋白质降解程度及肌节长度均低于对照组。【结论】肌原纤维蛋白磷酸化水平提高不利于羊肉肌原纤维蛋白的降解。另一方面,磷酸化水平可能通过对肌球蛋白轻链2的作用增强羊肉肌肉的收缩作用力,通过促进相邻原肌球蛋白的相互作用促进肌细丝收缩,影响肉的僵直进程和嫩化进程。     

Four-jointed is a Golgi kinase that phosphorylates a subset of cadherin domains

The atypical cadherin Fat acts as a receptor for a signaling pathway that regulates growth, gene expression, and planar cell polarity. Genetic studies in Drosophila identified the four-jointed gene as a regulator of Fat signaling. We show that four-jointed encodes a protein kinase that phosphorylates serine or threonine residues within extracellular cadherin domains of Fat and its transmembrane ligand, Dachsous. Four-jointed functions in the Golgi and is the first molecularly defined kinase that phosphorylates protein domains destined to be extracellular. An acidic sequence motif (Asp-Asn-Glu) within Four-jointed was essential for its kinase activity in vitro and for its biological activity in vivo. Our results indicate that Four-jointed regulates Fat signaling by phosphorylating cadherin domains of Fat and Dachsous as they transit through the Golgi.     

Inhibition of myosin light chain kinase by p21-activated kinase

p21-activated kinases (PAKs) are implicated in the cytoskeletal changes induced by the Rho family of guanosine triphosphatases. Cytoskeletal dynamics are primarily modulated by interactions of actin and myosin II that are regulated by myosin light chain kinase (MLCK)-mediated phosphorylation of the regulatory myosin light chain (MLC). p21-activated kinase 1 (PAK1) phosphorylates MLCK, resulting in decreased MLCK activity. MLCK activity and MLC phosphorylation were decreased, and cell spreading was inhibited in baby hamster kidney-21 and HeLa cells expressing constitutively active PAK1. These data indicate that MLCK is a target for PAKs and that PAKs may regulate cytoskeletal dynamics by decreasing MLCK activity and MLC phosphorylation.     

Proteomic screen finds pSer/pThr-binding domain localizing Plk1 to mitotic substrates

We have developed a proteomic approach for identifying phosphopeptide binding domains that modulate kinase-dependent signaling pathways. An immobilized library of partially degenerate phosphopeptides biased toward a particular protein kinase phosphorylation motif is used to isolate phospho-binding domains that bind to proteins phosphorylated by that kinase. Applying this approach to cyclin-dependent kinases (Cdks), we identified the polo-box domain (PBD) of the mitotic kinase polo-like kinase 1 (Plk1) as a specific phosphoserine (pSer) or phosphothreonine (pThr) binding domain and determined its optimal binding motif. This motif is present in known Plk1 substrates such as Cdc25, and an optimal phosphopeptide containing the motif disrupted PBD-substrate binding and localization of the PBD to centrosomes. This finding reveals how Plk1 can localize to specific sites within cells in response to Cdk phosphorylation at those sites and provides a structural mechanism for targeting the Plk1 kinase domain to its substrates.     

Endogenous substrate for cyclic AMP-dependent protein kinase in adrenocortical polyadenylated messenger ribonucleoproteins

An endogenous polysomal cyclic AMP-dependent protein kinase specifically phosphorylates a 150,000-dalton peptide bound to an adrenocortical polyadenylated messenger ribonucleoprotein complex. There is a possibility that this protein is a physiological substrate of cyclic AMP-dependent protein kinase and that the phosphorylation and dephosphorylation of this substrate may be important in the translation control of adrenal polyadenylated messenger RNA.     

MAP激酶在植物信号传递网络中的功能

促分裂素原活化蛋白激酶(mitogen-activated protein kinases,MAP激酶,MAPK)链是真核生物信号传递网络中的重要途径之一.MAPK链由3类蛋白激酶MAP3K-MAP2K-MAPK组成,通过依次磷酸化将上游信号传递至下游应答分子.本文主要阐述MAPK链在植物的逆境反应、抗病反应和激素调控等信号传递网络中的功能.     

Specific expression of a tyrosine kinase gene, blk, in B lymphoid cells

Several pathways of transmembrane signaling in lymphocytes involve protein-tyrosine phosphorylation. With the exception of p56lck, a tyrosine kinase specific to T lymphoid cells that associates with the T cell transmembrane proteins CD4 and CD8, the kinases that function in these pathways are unknown. A murine lymphocyte complementary DNA that represents a new member of the src family has now been isolated and characterized. This complementary DNA, termed blk (for B lymphoid kinase), specifies a polypeptide of 55 kilodaltons that is related to, but distinct from, previously identified retroviral or cellular tyrosine kinases. The protein encoded by blk exhibits tyrosine kinase activity when expressed in bacterial cells. In the mouse and among cell lines, blk is specifically expressed in the B cell lineage. The tyrosine kinase encoded by blk may function in a signal transduction pathway that is restricted to B lymphoid cells.     

A cell cycle phosphoproteome of the yeast centrosome

Centrosomes organize the bipolar mitotic spindle, and centrosomal defects cause chromosome instability. Protein phosphorylation modulates centrosome function, and we provide a comprehensive map of phosphorylation on intact yeast centrosomes (18 proteins). Mass spectrometry was used to identify 297 phosphorylation sites on centrosomes from different cell cycle stages. We observed different modes of phosphoregulation via specific protein kinases, phosphorylation site clustering, and conserved phosphorylated residues. Mutating all eight cyclin-dependent kinase (Cdk)-directed sites within the core component, Spc42, resulted in lethality and reduced centrosomal assembly. Alternatively, mutation of one conserved Cdk site within γ-tubulin (Tub4-S360D) caused mitotic delay and aberrant anaphase spindle elongation. Our work establishes the extent and complexity of this prominent posttranslational modification in centrosome biology and provides specific examples of phosphorylation control in centrosome function.     

植物MAPK级联途径及其功能研究进展

促分裂原活化蛋白激酶(Mitogen Actived Protein Kinase,MAPK)是一种蛋白激酶,蛋白激酶又称蛋白磷酸化酶,其可通过将ATP上的磷酸基团转移到底物蛋白质氨基酸残基上,来催化底物蛋白质磷酸化。MAPK级联途径广泛存在于真核生物中。植物中的MAPK级联途径与动物和酵母类似,都包括MAPKKK、MAPKK和MAPK 3种蛋白激酶。大量的研究表明,植物中的MAPK级联途径不仅能被多种生物与非生物胁迫所激活,同时也参与激素信号转导以及植物的生长发育进程。文章就植物中MAPK级联途径及其功能的研究情况进行了综述,并展望了相关研究的发展趋势。     

Activation by IKKalpha of a second, evolutionary conserved, NF-kappa B signaling pathway

In mammals, the canonical nuclear factor kappaB (NF-kappaB) signaling pathway activated in response to infections is based on degradation of IkappaB inhibitors. This pathway depends on the IkappaB kinase (IKK), which contains two catalytic subunits, IKKalpha and IKKbeta. IKKbeta is essential for inducible IkappaB phosphorylation and degradation, whereas IKKalpha is not. Here we show that IKKalpha is required for B cell maturation, formation of secondary lymphoid organs, increased expression of certain NF-kappaB target genes, and processing of the NF-kappaB2 (p100) precursor. IKKalpha preferentially phosphorylates NF-kappaB2, and this activity requires its phosphorylation by upstream kinases, one of which may be NF-kappaB-inducing kinase (NIK). IKKalpha is therefore a pivotal component of a second NF-kappaB activation pathway based on regulated NF-kappaB2 processing rather than IkappaB degradation.     

Polymorphic secreted kinases are key virulence factors in toxoplasmosis

The majority of known Toxoplasma gondii isolates from Europe and North America belong to three clonal lines that differ dramatically in their virulence, depending on the host. To identify the responsible genes, we mapped virulence in F(1) progeny derived from crosses between type II and type III strains, which we introduced into mice. Five virulence (VIR) loci were thus identified, and for two of these, genetic complementation showed that a predicted protein kinase (ROP18 and ROP16, respectively) is the key molecule. Both are hypervariable rhoptry proteins that are secreted into the host cell upon invasion. These results suggest that secreted kinases unique to the Apicomplexa are crucial in the host-pathogen interaction.     

Beta-adrenergic receptor kinase: primary structure delineates a multigene family

The beta-adrenergic receptor kinase (beta-ARK), which specifically phosphorylates only the agonist-occupied form of the beta-adrenergic and closely related receptors, appears to be important in mediating rapid agonist-specific (homologous) desensitization. The structure of this enzyme was elucidated by isolating clones from a bovine brain complementary DNA library through the use of oligonucleotide probes derived from partial amino acid sequence. The beta-ARK cDNA codes for a protein of 689 amino acids (79.7 kilodaltons) with a protein kinase catalytic domain that bears greatest sequence similarity to protein kinase C and the cyclic adenosine monophosphate (cyclic AMP)--dependent protein kinase. When this clone was inserted into a mammalian expression vector and transfected into COS-7 cells, a protein that specifically phosphorylated the agonist-occupied form of the beta 2-adrenergic receptor and phosphorylated, much more weakly, the light-bleached form of rhodopsin was expressed. RNA blot analysis revealed a messenger RNA of four kilobases with highest amounts in brain and spleen. Genomic DNA blot analysis also suggests that beta-ARK may be the first sequenced member of a multigene family of receptor kinases.     

Regulation of a heart potassium channel by protein kinase A and C

The enzymes adenosine 3',5'-monophosphate (cAMP)-dependent protein kinase (protein kinase A) and protein kinase C regulate the activity of a diverse group of cellular proteins including membrane ion channel proteins. When protein kinase A was stimulated in cardiac ventricular myocytes with the membrane-soluble cAMP analog 8-chlorphenylthio cAMP (8-CPT cAMP), the amplitude of the delayed-rectifier potassium current (IK) doubled when recorded at 32 degrees C but was not affected at 22 degrees C. In contrast, modulation of the calcium current (ICa) by 8-CPT cAMP was independent of temperature with similar increases in ICa occurring at both temperatures. Stimulation of protein kinase C by phorbol 12,13-dibutyrate also enhanced IK in a temperature-dependent manner but failed to increase ICa at either temperature. Thus, cardiac delayed-rectifier potassium but not calcium channels are regulated by two distinct protein kinases in a similar temperature-dependent fashion.     

An insulin-stimulated protein kinase similar to yeast kinases involved in cell cycle control

A protein kinase characterized by its ability to phosphorylate microtubule-associated protein-2 (MAP2), is thought to be an early intermediate in an insulin-stimulated phosphorylation cascade and in a variety of other mammalian cell responses to extracellular signals. A complementary DNA that encodes this protein serine-threonine kinase has been cloned, and the protein designated extracellular signal-regulated kinase 1 (ERK1). ERK1 has striking similarity to two protein kinases, KSS1 and FUS3, from yeast. The yeast kinases function in an antagonistic manner to regulate the cell cycle in response to mating factors. Thus, ERK1 and the two yeast kinases constitute a family of evolutionarily conserved enzymes involved in regulating the response of eukaryotic cells to extracellular signals.     

ATP regulates the phosphorylation and degradation of myofibrillar proteins in ground ovine muscle

Phosphorylation post-translational modification plays an important role in postmortem muscle quality traits. Adenosine triphosphate (ATP) is an energy source and a key substrate of phosphorylation which provides the phosphatase groups to proteins in the presence of protein kinases. However, in postmortem muscle, the effects of ATP content on phosphorylation are poorly studied. The study investigated the effect of ATP on protein phosphorylation and degradation in postmortem ovine muscle. The ground muscle with/without additional ATP were treated/control groups and stored at 25 and 4°C, respectively. The ATP content led to different changes of pH value between the ATP-treated and control groups. The phosphorylation level of myofibrillar proteins was higher (P<0.05) in ATP-treated group compared to the control group at both temperatures, which suggested that ATP played a vital role in postmortem protein phosphorylation. A slower degradation rate of µ-calpain, desmin and troponin T was observed in the ATP-treated group which showed that there was a negative relationship between ATP level and the degradation of proteins. These observations clearly highlighted the role of ATP on the development of meat quality by regulating the phosphorylation and degradation of myofibrillar proteins in postmortem ovine muscle.     

The protein kinase complement of the human genome

We have catalogued the protein kinase complement of the human genome (the "kinome") using public and proprietary genomic, complementary DNA, and expressed sequence tag (EST) sequences. This provides a starting point for comprehensive analysis of protein phosphorylation in normal and disease states, as well as a detailed view of the current state of human genome analysis through a focus on one large gene family. We identify 518 putative protein kinase genes, of which 71 have not previously been reported or described as kinases, and we extend or correct the protein sequences of 56 more kinases. New genes include members of well-studied families as well as previously unidentified families, some of which are conserved in model organisms. Classification and comparison with model organism kinomes identified orthologous groups and highlighted expansions specific to human and other lineages. We also identified 106 protein kinase pseudogenes. Chromosomal mapping revealed several small clusters of kinase genes and revealed that 244 kinases map to disease loci or cancer amplicons.     

着色与非着色苹果品种中磷酸化蛋白质的鉴定与分析

【目的】苹果着色是一个重要的质量性状,构建苹果磷酸化蛋白质组并进行鉴定与分析,了解在苹果着色过程中的蛋白质磷酸化,为进一步阐明苹果着色机理提供参考。【方法】以着色‘嘎拉’和非着色‘金冠’两个品种苹果果皮为试材提取总蛋白,用TiO₂富集磷酸化肽段,对富集到的磷酸化肽段进行高效液相色谱分离,利用质谱鉴定磷酸化肽段,采用Mascot2.2和Proteome Discoverer1.4（thermo）软件进行蛋白质查库鉴定,使用的数据库为Uniprot_Maloideae.fasta。对鉴定到的磷酸化肽段和蛋白质进行分析,找出着色与非着色苹果品种中有差异的磷酸化蛋白质及其修饰位点。【结果】在着色苹果品种中鉴定到1 323个蛋白质、3 339个肽段和225个磷酸化肽段,发现磷酸化蛋白质约200-225种;在非着色苹果品种中鉴定到569个蛋白质、1 152个肽段和128个磷酸化肽段,发现磷酸化蛋白质约117-128种。比较分析表明,43个磷酸化肽段仅在非着色苹果品种中发现,139个磷酸化肽段仅在着色苹果品种中发现,在着色苹果品种中有更多的蛋白质发生了磷酸化,其中质膜H⁺-ATPase在两个苏氨酸位点发生磷酸化,过敏原蛋白和两个蛋白激酶在丝氨酸位点发生磷酸化,3个转录因子、1个钾转运蛋白和1个受体激酶都发生磷酸化。在两个苹果品种鉴定出的蛋白质中,发生蛋白质磷酸化的位点主要是丝氨酸,其次是苏氨酸,在酪氨酸位点发生蛋白质磷酸化很少。蛋白质WD40和花青苷合成途径中的相关酶蛋白C4H、4CL、CHS、CHI、F3′H、FLS、LDOX和UFGT在着色过程中未发生磷酸化。在着色和非着色苹果品种中都存在MYBR转录因子,并且都发生了蛋白质磷酸化。【结论】在着色苹果品种中产生了一些特有的磷酸化蛋白质,其中包括已知与着色相关的质膜H⁺-ATPase,苹果着色可能受到蛋白质磷酸化的影响。     

Reduced MAP kinase phosphatase-1 degradation after p42/p44MAPK-dependent phosphorylation

The mitogen-activated protein (MAP) kinase cascade is inactivated at the level of MAP kinase by members of the MAP kinase phosphatase (MKP) family, including MKP-1. MKP-1 was a labile protein in CCL39 hamster fibroblasts; its degradation was attenuated by inhibitors of the ubiquitin-directed proteasome complex. MKP-1 was a target in vivo and in vitro for p42(MAPK) or p44(MAPK), which phosphorylates MKP-1 on two carboxyl-terminal serine residues, Serine 359 and Serine 364. This phosphorylation did not modify MKP-1's intrinsic ability to dephosphorylate p44(MAPK) but led to stabilization of the protein. These results illustrate the importance of regulated protein degradation in the control of mitogenic signaling.