First-order antiferromagnetic transitions of SrMn2P2 and CaMn2P2 single crystals containing corrugated-honeycomb Mn sublattices

SrMn₂P₂ and CaMn₂P₂ are insulators that adopt the trigonal CaAl₂Si₂-type structure containing corrugated Mn honeycomb layers. Magnetic susceptibility χ and heat capacity versus temperature T data reveal a weak first-order antiferromagnetic (AFM) transition at the Néel temperature TN=53(1) K for SrMn₂P₂ and a strong first-order AFM transition at TN=69.8(3) K for CaMn₂P₂. Both compounds exhibit isotropic and nearly T-independent χ(T≤TN), suggesting magnetic structures in which nearest-neighbor moments are aligned at ≈120° to each other. The ³¹P NMR measurements confirm the strong first-order transition in CaMn₂P₂ but show critical slowing down above TN for SrMn₂P₂, thus also evidencing second-order character. The ³¹P NMR measurements indicate that the AFM structure of CaMn₂P₂ is commensurate with the lattice whereas that of SrMn₂P₂ is incommensurate. These first-order AFM transitions are unique among the class of (Ca, Sr, Ba)Mn₂ (P, As, Sb, Bi)₂ compounds that otherwise exhibit second-order AFM transitions. This result challenges our understanding of the circumstances under which first-order AFM transitions occur.

The Mn-based 122-type pnictides AMn2Pn2 (A= Ca, Sr, Ba; Pn = P, As, Sb, Bi) have received attention owing to their close stoichiometric 122-type relationship to high-Tc iron pnictides. The undoped Mn pnictides are local-moment antiferromagnetic (AFM) insulators like the high-Tc cuprate parent compounds (1–3). The BaMn2Pn2 compounds crystallize in the body-centered tetragonal ThCr2Si2 structure as in AFe2As2 (A = Ca, Sr, Ba, Eu), whereas the (Ca,Sr)Mn2Pn2 compounds crystallize in the trigonal CaAl2Si2-type structure (4). Recently, density-functional theory (DFT) calculations for the 122 pnictide family have suggested that the trigonal 122 transition-metal pnictides that have the CaAl2Si2 structure might compose a new family of magnetically frustrated materials in which to study the potential superconducting mechanism (5, 6). It had previously been suggested on theoretical grounds that CaMn₂Sb₂ is a fully frustrated classical magnetic system arising from proximity to a tricritical point (7–9).The electrical resistivity ρ and heat capacity Cp versus temperature T of single-crystal CaMn₂P₂ were reported in ref. 10. The compound is an insulator at T = 0 and undergoes a first-order transition of some type at 69.5 K. The Raman spectrum of CaMn₂P₂ at T = 10 K showed new peaks compared to the spectrum at 300 K, whereas the authors’ single-crystal X-ray diffraction measurements showed no difference in the crystal structure at 293 and 40 K. They suggested that the results of the two types of measurements could be reconciled if a superstructure formed below 69.5 K (10). The authors’ magnetic susceptibility χ(T) measurements below 400 K revealed no evidence for a magnetic transition.Here we report the detailed properties of trigonal CaMn₂P₂ and SrMn₂P₂ (11) single crystals. We present the results of single-crystal X-ray diffraction (XRD), electrical resistivity ρ in the ab plane (hexagonal unit cell) versus temperature T, isothermal magnetization versus applied magnetic field M(H), magnetic susceptibility χ(T), heat capacity Cp(H,T), and ³¹P NMR measurements. We find from Cp(T), χ(T), and NMR that CaMn₂P₂ exhibits a strong first-order AFM transition at TN=69.8(3) K whereas SrMn₂P₂ shows a weak first-order transition at TN=53(1) K but with critical slowing down on approaching TN from above as revealed from NMR, a characteristic feature of second-order transitions. Thus, remarkably, the AFM transition in SrMn₂P₂ has characteristics of both first- and second-order transitions. The χ(T) data also reveal the presence of strong isotropic AFM spin fluctuations in the paramagnetic (PM) state above TN up to our maximum measurement temperatures of 900 and 350 K for SrMn₂P₂ and CaMn₂P₂, respectively. This behavior likely arises from spin fluctuations associated with the quasi–two-dimensional nature of the Mn spin layers (12) together with possible contributions from magnetic frustration. Our single-crystal XRD data at room temperature and high-resolution synchrotron XRD data at T = 20 K for SrMn₂P₂ and CaMn₂P₂ demonstrate conclusively that there is no structure change of either compound on cooling below their respective TN.Our studies of SrMn₂P₂ and CaMn₂P₂ thus identify the only known members of the class of materials with general formula AMn2Pn2 containing Mn2+ spins S = 5/2 that exhibit first-order AFM transitions, where A = Ca, Sr, or Ba and the pnictogen Pn= P, As, Sb, or Bi. In particular, only second-order AFM transitions are found in CaMn2As2 (13), SrMn2As2 (13–15), CaMn2Sb2 (8, 9, 16–19), SrMn2Sb2 (16, 19), and CaMn2Bi2 (20).     

P2y1 and P2y2 receptor-operated Ca2+ signals in primary cultures of cardiac microvascular endothelial cells

Intracellular Ca2+ signals elicited by nucleotide agonists were investigated in primary cultures of rat cardiac microvascular endothelial cells using the fura-2 technique. UTP increased the intracellular [Ca2+] in 94% of the cells, whereas 2MeSATP was active in 32%. The rank order of potency was ATP = UTP > 2MeSATP and the maximal response to 2MeSATP was lower compared to UTP and ATP. ATP and UTP showed strong homologous and heterologous desensitization. ATP fully inhibited the 2MeSATP response, while UTP abolished 2MeSATP-elicited transients in 25% of cells. 2MeSATP did not desensitize the UTP or ATP response. Adenosine 2',5'-diphosphate inhibited the response to 2MeSATP, while it did not modify the response to ATP and UTP. 2MeSATP was more sensitive to suramin than UTP and ATP. These results indicate that P(2Y1) and P(2Y2) receptors may be coexpressed in CMEC. Nucleotide-induced Ca2+ signals lacked a sustained plateau and were almost independent from extracellular Ca2+. ATP and UTP elicited Ca2+ transients longer than 2MeSATP-evoked transients. The kinetics of Ca2+ responses was not affected by bath solution stirring or ectonucleotidase inhibition. Furthermore, the nonhydrolyzable ATP analogue AMP-PNP induced Ca2+ signals similar to those elicited by ATP and UTP. These results suggest that the distinct kinetics of nucleotide-evoked Ca2+ responses do not depend on the activity of ectonucleotidases or ATP autocrine stimulation. The possibility that Ca2+ signals with different time courses may modulate different cellular responses is discussed.     

P2Y6 and vascular inflammation

In this issue of Blood, Riegel and colleagues demonstrate that inflammatory stimuli induce the expression of the P2Y6 receptor on the vascular endothelium where it serves to enhance systemic inflammatory responses.     

Evidence for separate calcium-signaling P2T and P2U purinoceptors in human megakaryocytic Dami cells

Recently (J Pharmacol Exp Ther 261:580, 1992), we have shown that K562 leukemia cells express a calcium-signaling purinoceptor with characteristics of the P2T receptor subtype for adenosine diphosphate (ADP) previously found only in platelets. Because these results suggested that the P2T receptor may be an early marker for megakaryocytic differentiation, we studied whether this calcium- signaling receptor is also expressed in Dami cells, a human megakaryocytic leukemia cell line. Here we report evidence that Dami cells express a P2T receptor for ADP. The calcium response EC50 values for ADP, 2-methylthioadenosine diphosphate (2-MeS-ADP), and adenosine 5'-O-(2-thiodiphosphate) (ADP beta S) in Dami cells are 0.4 mumol/L, 0.04 mumol/L, and 2 mumol/L, respectively, which approximate the potencies of these agonists in K562 cells and in platelets. The platelet P2T receptor antagonists 2-methylthioadenosine triphosphate (2- MeS-ATP), and 2-chloroadenosine triphosphate (2-Cl-ATP) were surprisingly potent agonists at the P2T receptor in both Dami and K562 cells. Dami cells, unlike K562 cells and platelets, also respond to adenosine triphosphate (ATP) and uridine triphosphate (UTP) with an increase in intracellular calcium. Adenosine monophosphate (AMP) is an effective antagonist of the response to ADP, 2-MeS-ADP, ADP beta S, 2- MeS-ATP, and 2-Cl-ATP, but not to ATP and UTP. The responses to maximal concentrations of UTP in combination with either ADP, 2-MeS-ADP, ADP beta S, or 2-MeS-ATP are additive. In contrast, ADP in combination with either 2-MeS-ADP, ADP beta S, 2-MeS-ATP, or 2-Cl-ATP are not additive. UTP desensitized Dami cells to ATP but not to ADP, 2-MeS-ADP, ADP beta S, or 2-MeS-ATP. Addition of ATP after UTP desensitization antagonized subsequent responsiveness to ADP. The data suggest that the receptor for ADP may be a unique P2T subtype, and the receptor for ATP and UTP is distinct from that of ADP and is most characteristic of the P2U (nucleotide) receptor subtype. Activation of either the P2T or P2U receptor causes a rapid generation of inositol trisphosphate in Dami cells.     

Enzymatic Utilization of P1-Di-N-acetylchitobiosyl P2-Dolichyl Pyrophosphate and Its Chemical Synthesis

Fully acetylated chitobiose was treated with phosphoric acid to give a mixture of products from which 2-acetamido-4-O-(2-acetamido-3,4,6-tri-O-acetyl-2-deoxy-beta- D-glucopyranosyl)-3,6-di-O-acetyl-2-deoxy-alpha,beta- D-glucopyranosyl phosphate (Ac(3)GlcNAc-Ac(2)GlcNAc-P) was isolated by preparative thin layer chromatography. Treatment of this compound with P(1)-diphenyl P(2)-dolichyl pyrophosphate gave an acetylated pyrophosphate diester, which was purified chromatographically and deacetylated. The product, P(1)-di-N-acetylchitobiosyl P(2)-dolichyl pyrophosphate (Dol-P-P-GlcNAc-GlcNAc), was readily separated from P(1)-2-acetamido-2-deoxy-alpha-D-glucopyranosyl P(2)-dolichyl pyrophosphate (Dol-P-P-GlcNAc) by thin layer chromatography in several solvent systems. Addition of this compound to human lymphocyte membrane preparations led to the formation of a mannose-containing derivative which appears to be an oligosaccharide phospholipid, as judged by its behavior on DEAE-cellulose chromatography and by its hydrolysis to give an oligosaccharide containing more than four monosaccharide units.     

P2Y1 and P2Y12 receptors for ADP desensitize by distinct kinase-dependent mechanisms

Adenosine 5'-diphosphate (ADP) plays a central role in regulating platelet function by the activation of the G protein-coupled receptors P2Y(1) and P2Y(12). Although it is well established that aggregation responses of platelets to ADP desensitize, the underlying mechanisms involved remain unclear. In this study we demonstrate that P2Y(1)- and P2Y(12)-mediated platelet responses desensitize rapidly. Furthermore, we have established that these receptors desensitize by different kinase-dependent mechanisms. G protein-coupled receptor kinase (GRK) 2 and GRK6 are both endogenously expressed in platelets. Transient overexpression of dominant-negative mutants of these kinases or reductions in endogenous GRK expression by the use of specific siRNAs in 1321N1 cells showed that P2Y(12), but not P2Y(1), desensitization is mediated by GRKs. In contrast, desensitization of P2Y(1), but not P2Y(12), is largely dependent on protein kinase C activity. This study is the first to show that both P2Y(1) and P2Y(12) desensitize in human platelets, and it reveals ways in which their sensitivity to ADP may be differentially and independently altered.     

Overview of the P2 receptors

The release of nucleotides in extracellular fluids can result from cell necrosis, exocytosis of secretory granules (such as platelet dense granules), or efflux through membrane channels. In addition, recent evidence suggests that vesicular trafficking is an important pathway of nucleotide release. Once in the extracellular fluids, they are rapidly degraded by ectonucleotidases, such as CD39, that play a key role in neutralizing the platelet aggregatory action of adenosine diphosphate (ADP), and act on two families of receptors: the ionotropic P2X receptors and the G-protein-coupled P2Y receptors. The family of P2X receptors encompasses seven genes. Currently, there are eight genuine P2Y receptors that can be subdivided into two structurally distinct subfamilies. Whereas P2X receptors are receptors of ATP, the different P2Y receptors are activated by distinct nucleotides, diphosphates or triphosphates, or purines or pyrimidines, some of them being conjugated to sugars. The study of knockout mice has demonstrated that P2X receptors play important roles in the neurogenic control of smooth muscle contraction, in pain and visceral perception, and in macrophage functions. The phenotype of P2Y null mice so far is more restricted: inhibition of platelet aggregation to ADP and increased bleeding time in P2Y (1)(-/-) and P2Y (12)(-/-) mice and lack of epithelial responsiveness to nucleotides in airways (P2Y (2)(-/-)) and intestine (P2Y (4)(0/-)).     

P2嘌呤受体与胃肠感觉的研究进展

P2受体是嘌呤受体,它在胃肠道的感觉中发挥着重要的作用,下面就P2受体在胃肠道的分布、感觉功能及其与相关疾病的关系做一综述.     

P2RY1 and P2RY12 polymorphisms and on-aspirin platelet reactivity in patients with coronary artery disease

Introduction: Association of P2RY1 and P2RY12 polymorphisms with on‐aspirin platelet reactivity was investigated. Materials and methods: Platelet reactivity was assessed by the light transmission aggregometry and TxB₂ assay in 423 patients with coronary artery disease (CAD) on aspirin. High residual platelet reactivity (RPR) was defined by ≥20% and ≥70% maximal aggregation stimulated with 0.5 mg/mL arachidonic acid (AA) and 10 μm ADP, respectively. Moderate RPR was considered aggregation ≥20% with AA, ≥70% with ADP, or ≥1 ng/mL stimulated TxB₂. Fourteen P2RY1 and 35 P2RY12 single nucleotide polymorphisms (SNPs) were genotyped. Results: High RPR was detected in 24% of the patients. Moderate RPR was observed in 31% with AA, 57% with 5 μm ADP, and 82% with 10 μm ADP. Stimulated TxB₂ was ≥1 ng/mL in 23% of patients. P2RY12 SNP rs9859538 was associated with high RPR (OR = 2.16, 95% CI = 1.24–3.75, P‐value = 0.004). Four P2RY12 SNPs, rs1491974, rs10513398, rs3732765, and rs10935841, showed association with moderate RPR (OR = 1.79–2.94, P‐value = 0.04–0.028), while five, rs7615865, rs1388623, rs1388622, rs7634096, and rs7637803, were associated with low RPR (OR = 0.50–0.55, P‐value = 0.008–0.026), following ADP stimulation. TxB₂ level <1 ng/mL was linked to five P2RY1 SNPs, rs1439010, rs1371097, rs701265, rs12497578, and rs2312265 (OR = 0.36–0.54, P‐value = 0.003–0.039). Conclusions: Polymorphisms in P2RY1 and P2RY12 are associated with on‐aspirin platelet reactivity in patients with CAD.     

包含P2X3亚基的受体与内脏高敏感性

三磷酸腺苷(ATP)门控阳离子通道型受体P2X31995年克隆成功,特别在小直径伤害性感觉神经元中高表达。越来越多的研究表明,包含P2X3亚基的同聚体P2X3及异聚体P2X2/3在介导内脏伤害性信息传递过程中起重要作用,有可能成为功能性胃肠疾病新的治疗靶点。     

P2X7受体与糖尿病视网膜病变

P2X7受体是一种重要的凋亡调控受体,是嘌呤受体家族中的一员,也是ATP活化的配体门控离子通道的调节者.它在中枢和外周神经系统中对介导兴奋性神经递质起重要作用.P2X7受体广泛表达于视网膜多种细胞表面.研究显示,P2X7受体在糖尿病视网膜病变中过度激活,参与糖尿病视网膜病变的发生及发展.一方面,P2X7受体过度激活所致的嘌呤血管毒性,可导致视网膜血流减少和血管功能的紊乱;另一方面,P2X7受体活化可导致大量炎性因子的产生,引起局部炎性细胞浸润,形成血管炎性微环境,构成糖尿病视网膜病变发生、发展的病理生理基础.     

Impact of ticagrelor on P2Y1 and P2Y12 localization and on cholesterol levels in platelet plasma membrane

Ticagrelor is an antiplatelet agent that inhibits platelet activation via P2Y12 antagonism. There are several studies showing that P2Y12 needs lipid rafts to be activated, but there are few data about how ticagrelor impacts lipid raft organization. Therefore, we aimed to investigate how ticagrelor could impact the distribution of cholesterol and consequently alter the organization of lipid rafts on platelet plasma membranes. We identified cholesterol-enriched raft fractions in platelet membranes by quantification of their cholesterol levels. Modifications in cholesterol and protein profiles (Flotillin 1, Flotillin 2, CD36, P2Y1, and P2Y12) were studied in platelets stimulated by ADP, treated by ticagrelor, or both. In ADP-stimulated and ticagrelor-treated groups, we found a decreased level of cholesterol in raft fractions of platelet plasma membrane compared to the control group. In addition, the peak of cholesterol in different experimental groups changed its localization on membrane fractions. In the control group, it was situated on fraction 2, while in ADP-stimulated platelets, it was located in fractions 3 to 5, and in fraction 4 in ticagrelor-treated group. The proteins studied also showed changes in their level of expression and localization in fractions of plasma membrane. Cholesterol levels of plasma membranes have a direct role in the organization of platelet membranes and could be modified by stimulation or drug treatment. Since ticagrelor and ADP both changed lipid composition and protein profile, investigating the lipid and protein composition of platelet membranes is of considerable importance as a focus for further research in anti-platelet management.     

尖锐湿疣组织中P16 P63 NF-kBp65及TRAIL-R2的表达

目的研究P16、P63、核转录因子kBp65(NF-kBp65)及肿瘤坏死因子相关凋亡诱导配体受体2(TRAIL-R2)在尖锐湿疣组织中的表达。方法采用免疫组织化学SABC法和图像分析系统检测30例尖锐湿疣患者皮损中,15例正常人皮肤(包皮)组织中,P16、P63、NF-kBp65及TRAIL-R2的表达。结果(1)P63、NF-kBp65、TRAIL-R2在尖锐湿疣组织中的表达均高于正常皮肤组织,差异有统计学意义(P<20.05);(2)P16在尖锐湿疣组织中的表达较正常包皮组织中高,但无统计学意义(P>0.05)。结论在尖锐湿疣的发生发展过程中,P63、NF-kBp65、TRAIL-R2起到一定的作用,共同影响细胞凋亡,促进表皮细胞的增殖。