大鼠急性肺栓塞后SMP-30表达下降及其对细胞凋亡的影响

目的：研究大鼠急性肺栓塞模型肺组织中衰老标记蛋白质30(SMP-30)的表达变化及其对Fas诱导的细胞凋亡的影响。方法:建立大鼠急性肺栓塞模型，分别在急性肺栓塞后1、8、24和48 h进行支气管肺泡灌洗，然后开胸取出肺组织。常规提取肺组织的总RNA和总蛋白，以正常组为对照，采取半定量RT-PCR的方法研究SMP-30在mRNA水平表达的变化；采用Western blotting方法进一步验证SMP-30在蛋白水平表达的变化；采用免疫组织化学方法检测大鼠肺组织中SMP-30以及肺泡巨噬细胞中IL-8在肺栓塞前后表达的变化及其组织分布情况；采用TUNEL法研究急性肺栓塞后组织细胞的凋亡情况；最后采用ELISA法检测急性肺栓塞后肺泡灌洗液中sFasL的浓度变化。结果:在大鼠急性肺栓塞后的不同时点，SMP-30的mRNA水平和蛋白水平均逐渐降低，在24和48 h下降最为明显。免疫组化研究表明SMP-30主要分布在支气管黏膜上皮细胞和肺泡上皮细胞，急性肺栓塞后SMP-30在上述细胞内的表达均明显降低。TUNEL染色发现随着SMP-30表达的降低，肺组织内出现明显的细胞凋亡现象，同时肺泡灌洗液中sFasL的浓度升高，肺泡巨噬细胞内IL-8的表达也明显升高。结论:大鼠急性肺栓塞后肺组织内SMP-30的表达明显降低，可能促进Fas－FasL细胞凋亡系统的活化。     

Megalencephaly syndromes associated with mutations of core components of the PI3K‐AKT–MTOR pathway: PIK3CA,PIK3R2, AKT3, and MTOR

Megalencephaly (MEG) is a developmental abnormality of brain growth characterized by early onset, often progressive, brain overgrowth. Focal forms of megalencephaly associated with cortical dysplasia, such as hemimegalencephaly and focal cortical dysplasia, are common causes of focal intractable epilepsy in children. The increasing use of high throughput sequencing methods, including high depth sequencing to more accurately detect and quantify mosaic mutations, has allowed us to identify the molecular etiologies of many MEG syndromes, including most notably the PI3K‐AKT‐MTOR related MEG disorders. Thorough molecular and clinical characterization of affected individuals further allow us to derive preliminary genotype–phenotype correlations depending on the gene, mutation, level of mosaicism, and tissue distribution. Our review of published data on these disorders so far shows that mildly activating variants (that are typically constitutional or germline) are associated with diffuse megalencephaly with intellectual disability and/or autism spectrum disorder; moderately activating variants (that are typically high‐level mosaic) are associated with megalencephaly with pigmentary abnormalities of the skin; and strongly activating variants (that are usually very low‐level mosaic) are associated with focal brain malformations including hemimegalencephaly and focal cortical dysplasia. Accurate molecular diagnosis of these disorders is undoubtedly crucial to more optimally treat children with these disorders using PI3K‐AKT–MTOR pathway inhibitors.     

IL-15 and IL-15Rα gene deletion: Effects on T lymphocyte trafficking and the microglial and neuronal responses to facial nerve axotomy

IL-15 is a potent T cell chemoattractant, and this cytokine and its unique α subunits, IL-15Rα, can modify immune cell expression of several T cell chemokines and their receptors. Facial nerve axotomy in mice leads to T cell migration across an intact blood–brain-barrier (BBB), and under certain conditions T cells can provide neuroprotection to injured neurons in the facial motor nucleus (FMN). Although chemokines and chemoattractant cytokines are thought to be responsible for T cell migration to the injured cell bodies, data addressing this question are lacking. This study tested the hypothesis that T cell homing to the axotomized FMN would be impaired in knockout (KO) mice with the IL-15 and IL-15Rα genes deleted, and sought to determine if microglial responsiveness and motoneuron death are affected. Both IL-15KO and IL-15RαKO mice exhibited a marked reduction in CD3⁺ T cells and had fewer MHC2⁺ activated microglia in the injured FMN than their respective WT controls at day 14 post-axotomy. Although there was a relative absence of T cell recruitment into the axotomized FMN in both knockout strains, IL-15RαKO mice had five times more motoneuron death (characterized by perineuronal microglial clusters engulfing dead motoneurons) than their WT controls, whereas dead neurons in IL-15KO did not differ from their WT controls. Further studies are needed to dissect the mechanisms that underlie these observations (e.g., central vs. peripheral immune contributions).     

Growth of diploid cells from breast cancers

Cell cultures were derived from normal and cancerous breast tissues and from metastases by methods that selected for relatively adherent epithelial aggregates. Karyotypic analyses of first or second passage cultures yielded predominantly normal diploid cells. Nonclonal aberrations were more common in tumor-derived than in normal cultures. Three of the cultures that originated from metastases were characterized by abnormal clones. These results support observations based on DNA content, which indicate that a considerable fraction of breast cancers are composed predominantly of diploid cells. They differ greatly from chromosomal findings in long-term cultures of tumor effusions and thus emphasize the karyotypic diversity that can be found in tumors from a single tissue of origin--the breast.     

Quantitative determination of anti-dsDNA antibodies and antibody/dsDNA stoichiometries in prepared,soluble complement-fixing antibody/dsDNA immune complexes

We have investigated quantitatively the complement-mediated binding of prepared, soluble ¹²⁵I-7S IgG antibody/³H-dsDNA immune complexes to human red blood cells (RBCs). We have performed these studies by using a detailed modification of the RBC-CF assay [Pedersen et al., J. Immun. Meth. 38, 2692–2280 (1980)] which now allows for the simultaneous measurement of both ³H-DNA and ¹²⁵I-binding to the cells. Our results indicate that, in the case of three SLE patients, their anti-dsDNA antibody titers are sufficiently high that a small fraction of their ¹²⁵I-7S IgG antibodies (ca 0.1–0.2%) can be identified as specifically anti-dsDNA. We have also used an indirect method (with ¹²⁵I-labelled rabbit anti-human IgG) for the determination of IgG anti-dsDNA antibodies in complement-fixing antibody/dsDNA immune complexes that bind to RBCs, and the results of these measurements are in reasonable agreement with the direct binding experiments. These studies have also allowed us to estimate the antibody/DNA stoichiometries in complement-fixing immune complexes. The results of these experiments may provide a useful standard for the analysis of monoclonal anti-dsDNA antibodies.     

Variant Philadelphia chromosome translocations in two patients with chronic myelogenous leukemia

Two patients with chronic myelogenous leukemia and new variant Philadelphia chromosome translocations are reported. In one case, a 41-year-old male, a 10;22 translocation was found in all bone marrow cells examined. Furthermore, the Y chromosome was missing in 90% of the analyzed metaphase cells. In the second patient, a 22-year-old male, all the marrow cells contained a complex rearrangement involving chromosomes No. 2, 9, and 22.     

Size distribution and In vitro translation of the RNAs isolated from turnip yellow mosaic virus nucleoproteins

Purified preparations of TYMV contain a number of minor nucleoprotein components distinguishable on the basis of their density in CsCl gradients (R. E. F. Matthews, Virology12, 521–539, 1960). When analysed by polyacrylamide-gel eletrophoresis, the RNA from each of these various components was found to consist of a characteristic set of molecular-weight species. Full-size RNA (2 × 10⁶ daltons) was present only in nucleoproteins B₁ and B₂. Nucleoproteins B₀, B₀₀, and B₀₀₀ contained RNAs ranging in size from approx 1.3 to 0.28 × 10⁶ daltons. The 0.28 × 10⁶-dalton RNA species was detectable in all nucleoprotein fractions, but was a significant proportion of the RNAs of B₀₀₀ and B₀₀. Translation of the RNA from each of the nucleoproteins in the wheat germ cell-free protein synthesizing system yielded essentially similar patterns of polypeptides which ranged in size from 5000 to 70,000 daltons. The major radioactive product migrated on SDS-polyacrylamide gels to the same position as TYMV coat protein. The data suggest that the 0.28 × 10⁶-dalton RNA component is the cistron for coat protein, and that it and other RNAs associated with TYMV infection are encapsidated.     

HOME AND LABORATORY DREAMS COLLECTED UNDER UNIFORM SAMPLING CONDITIONS

Twelve young-adult males spent two nonconsecutive nights at the laboratory (L) and two at home (H), six in the order LHHL and six in the order HLLH. Dreams were collected under uniform sampling conditions in both settings: S was awakened by an alarm clock at 6:30 a.m. and reported any dreams he could remember into a tape recorder. Twenty dream reports were collected in the laboratory, and 18 at home. Dream reports were rated by two judges on the six dimensions isolated by Hauri et al.'s factor analysis of dream ratings. Results showed no significant differences between home and laboratory in percentage of recall, median dream word counts, and dream ratings for Vivid Fantasy, Unpleasantness, Active Participation, and Sex. Home dreams were judged to contain more Verbal Aggression (p < .02) and Physical Aggression (p < .08). It was concluded that, although impulse-related content may be more likely to occur in home dreams than in laboratory dreams, the basic dream processes of imagination, distortion, dramatization, etc., are the same in both settings.     

支气管肺炎患儿治疗前后血清SIL-2R和白三烯测定的临床意义

目的：探讨了血清可溶性白细胞介素-2受体（SIL-2R）和半胱氨酰白三烯（LTS）水平在支气管肺炎患儿治疗前后的变化及意义。方法：应用ELISA对35例支气管肺炎患儿进行了血清SIL-2R和LTS测定，并与30例正常儿作比较。结果：支气管肺炎患儿在治疗前血清SIL-2R和LTS水平非常显著地高于正常儿组（P〈0.01）。治疗后2周后血清SIL-2R和LTS水平与正常儿比较无显著性差异（P〉0．05）。结论：检测支气管肺炎患儿血清中SIL-2R和LTS水平可作为病情预后判断的重要指标。     

通痹灵对于IL-2及其受体α链影响的体内外研究

从体内体外两个方面 ,研究通痹灵对于CIA大鼠关节滑膜原代细胞分泌IL 2 ,以及通痹灵总碱对于IL 2受体α链CD2 5表达的影响。体内实验采用CIA大鼠动物模型。容积法测量足肿胀度 ,原代滑膜细胞培养、放免法检测培养液上清 ,观察通痹灵对滑膜内IL 2的影响 ;体外实验 ,分离大鼠淋巴细胞 ,佛波醇酯 (PDB )或刀豆蛋白 (ConA )体外刺激 ,双色免疫荧光标记 ,流式细胞仪检测 ,观察通痹灵总碱对CD3+CD2 5 +表达的影响。结果是体内实验 ,通痹灵高剂量可明显减轻CIA大鼠的足肿胀度 ,与MTX比较无显著性差异 (P >0 0 5 ) ,通痹灵高、低剂量可明显抑制CIA大鼠滑膜内IL 2的合成 (P <0 0 1) ;体外实验 ,通痹灵总碱显著抑制ConA刺激下的CD3+CD2 5 +的表达 ,而对PDB加ionomycin没有明显作用。提示通痹灵可以通过抑制IL 2合成及ConA激活的IL 2受体α链CD2 5信号转导通路 ,减轻局部关节的炎症 ,为其用于类风湿性关节炎的治疗提供了实验依据