外围由小分子修饰的树枝状聚酰胺的合成及其荧光性能研究

合成了1－5代外围由小分子荧光体修饰的树枝状聚酰胺，通过红外，紫外，核磁等表征了其结构，并对其荧光性能进行了研究，修饰后的固体产物的荧光较修饰前粘稠体产物的荧光强得多，树枝状高分子荧光受组分比，代数，溶液浓度，溶剂等因素的影响，有机硅对树状高分子的端氨基与3，5二羟基苯甲酸按1／1摩尔比反应时，其产物荧光最强，对于端氨基与3，5－二羟基苯甲酸摩尔比为1／1的不同代树枝状聚酰胺而言，2代产物荧光最强。     

母血中胎儿有核红细胞的荧光原位杂交法在产前诊断中的可行性探讨

探讨荧光原位杂交法（FISH）对母血中胎儿有核红细胞（NRBC）进行无创性产前诊断的可行性。20例孕龄15-20周的孕妇外周血经不连续密度梯度离心、制片、显微镜下识别并共计数NRBC及定位，然后行Y染色体的FISH检测。结果发现10例孕男性胎儿的孕妇外周血细胞涂片中每例均有阳性杂交信号出现；阳性率为60％（24/40）。10例孕女性胎儿的孕妇外周血细胞涂片中1例出现阳性杂交信号；阴性率为95％（38/40），假阳性率仅为5％（2/40）。结果提示FISH法对于用母血中分离到的胎儿细胞进行染色体异常的无创性产前遗传学检查具有重要意义。     

用荧光原位杂交技术快速诊断孕早期胚胎染色体数目异常

目的探讨荧光原位杂交(FISH)技术在快速产前诊断孕早期胚胎染色体数目异常中的价值.方法采用13,18,21,X和Y染色体特异性DNA探针,对46例孕47～65 d高危孕妇的绒毛间期细胞进行FISH检测,同时行常规染色体核型分析平行诊断.结果与染色体核型分析结果一致的染色体数目正常43例,异常3例(47,XY 21;47,XY 18和45,X).3例异常核型胚胎经治疗性流产后再分别对其绒毛行常规染色体核型分析,结果与产前诊断相符.结论FISH技术用于产前诊断孕早期胚胎染色体数目异常具有快速、准确等优点.     

间期荧光原位杂交检测核心结合因子相关急性白血病的初步研究

目的应用间期荧光原位杂交技术(I-FISH)检测初诊急性白血病患者中核心结合因子(CBF)受累的染色体异常情况并对治疗后患者的微小残留病(MRD)进行监测,同时对I-FISH与常规染色体G显带的灵敏度进行比较。方法在骨髓形态学初筛的基础上,应用常规染色体G显带技术对15例急性髓系白血病(AML)进行核型分析,应用I-FISH对患者可能受累的CBF相关靶基因进行检测,其中7例患者治疗后进行了MRD监测。结果(1)正常对照组中,CYTOCELL公司提供的3种探针(AML1/ETO易位探针、MYH11基因断裂点双色探针和ETV6/AML1易位探针)的正常分界值分别为4.13%、1.95%和2.12%。(2)常规染色体G显带分析,15例患者中有6例伴有潜在累及CBF基因的染色体异常,其中8例AML-M2中5例伴t(8;21),2例AML-M4EO中1例伴inv(16),5例儿童B系急性淋巴细胞白血病(B-ALL)未检出相应的异常。I-FISH检测15例患者发现有12例累及CBF基因,其中8例AML-M2患者均为AML1/ETO融合基因(+),2例AML-M4EO病人CBFβ/MYH11融合基因均为(+),5例儿童B-ALL中2例ETV6/AML融合基因(+)。(3)3例AML-M2患者中2例MRD阳性;2例M4E0患者治疗后MRD监测结果均阴性;2例B-ALL患者1例阴性,1例阳性。结论I-FISH较常规染色体G显带技术能够更灵敏地检测出累及CBF的急性白血病,在初诊时联合应用这两种     

Studies on monoclonal anti-isotypic and anti-idiotypic antibodies against leukemia and myeloma: IV modulation of membrane fluidity of leukemic cell lines and tonsillar cell stimulated with McAbs

Summary In this study the technique of labelling the cell membrane with DPH fluorescence polarization was used to observe the membrane fluidity of B lymphocytic cell lines and tonsillar cells from healthy persons; the modulation effect on membrane-fluidity induced by McAbs against isotypic and idiotypic determinants of IgM from patients with leukemia was studied as well. The expression of the corresponding isotypic and idiotypic determinants of IgM on the cell membrane was determined. The results show that the membrane fluidity of leukemic cell lines is remarkably higher than that of tonsillar cells from healthy persons, and McAbs against isotypic determinants of leukemic IgM can enhance the membrane fluidity of all kinds of cells mentioned above. However, the anti-idiotypic monoclonal antibody increased only the membrane fluidity of leukemic cell lines. These results indicated that there was a close relationship between the effect of McAbs on cell membrane fluidity and the expression of corresponding isotypic and idiotypic determinants of IgM on the cell membrane.     

苯并恶唑类化合物的研究——Ⅰ.化合物的合成及光物理性能

合成了四种结构类型的苯并恶唑化合物共15个:测试了它们的红外吸收光谱,以及它们在DMF中的紫外吸收、荧光发射和激光发射光谱。苯基取代物的荧光量子产率在0.64～0.66,无激光性能。其余的化合物荧光量子产率都大于0.70,在最大吸收波长下的激光转换效率为2.5～5.9%。     

Monitoring myocardial reperfusion injury with NADH fluorometry.

Using NADH fluorometry to monitor myocardial metabolism, the mechanism of reperfusion injury was investigated after the delivery of an experimental reperfusate. Using an isolated working heart preparation, rat hearts underwent 15 min of global ischemia at 37 degrees C. Following the ischemic insult, an oxygenated enriched reperfusion solution was given for 5 min. The hearts were then returned to a working state and aortic flow recorded to evaluate recovery. NADH levels were monitored throughout the experiment with a fluorometer and glycogen, AMP, ADP, and ATP were measured biochemically pre- and postischemia, after reperfusion and after recovery. In this study, reperfusion injury was best abated by an enriched reperfusate. Our results indicate the mechanism for this amelioration is not high-energy phosphate replenishment. Rather, as indicated by NADH fluorescence, the hearts attain an intermediate level of metabolism that permits glycogen to be restored and functional recovery to be improved.     

Triploid origin of the gibel carp as revealed by 5S rDNA localization and chromosome painting

5S ribosomal DNA (rDNA) was isolated and sequenced from the gibel carp Carassius auratus gibelio with 162 chromosomes and crucian carp Carassius auratus with 100 chromosomes, and fluorescent probes for chromosome localization were prepared to ascertain the ploidy origin and evolutionary relationship between the two species. Using fluorescence in-situ hybridization (FISH), major 5S rDNA signals were localized to the short arms of three subtelocentric chromosomes in the gibel carp and to the short arms of two subtelocentrics in the crucian carp. In addition, some minor signals were detected on other chromosomes of both species. Simultaneously, six chromosomes were microdissected from the gibel carp metaphase spreads using glass needles, and the isolated chromosomes were amplified in vitro by degenerate oligonucleotide primed-polymerase chain reaction (DOP-PCR). Significantly, when the DOP-PCR-generated probes prepared from each single chromosome were hybridized, three same-sized chromosomes were painted in each gibel carp metaphase, whereas only two painted chromosomes were observed in each crucian carp metaphase spread. The data indicate that gibel carp is of triploid origin in comparison with diploid crucian carp.     

激光荧光检测仪对乳牙合面患龋敏感位点的流行病学研究

目的：定量分析乳牙合面的龋病敏感点位，为指导临床预防和治疗龋病提供依据。方法：采用激光荧光检测仪（DIAGNOdent）检测156名5～6岁儿童共561颗患龋的乳磨牙合面，记录合面龋坏最严重的位点。结果：在上颌第2乳磨牙中，龋坏最严重的位点有60．1％发生在远中窝。在下颌第2乳磨牙中，龋坏最严重的位点有51．2％发生在舌沟；而在下颌第1乳磨牙中，龋坏最严重的位点则易发生在远中窝，占该牙记录位点的34．9％。结论：不同的牙合面患龋严重部位具有统计学规律，提示这些位点是龋坏容易发生和发展的地方，是临床上预防和治疗不可忽略的重要部位。     

Mapping the Distribution of the Telomeric Sequence (T2AG3) n in the 2n = 14 Ancestral Marsupial Complement and in the Macropodines (Marsupialia: Macropodidae) by fluorescence in situ hybridization

In this study we test the theory that the presence of the conserved vertebrate telomeric sequence (T(2)AG(3))(n) at the centromeres of Australian marsupial 2n = 14 complements is evidence that these karyotypes are recently derived, which is contrary to the generally held view that the 2n = 14 karyotype is ancestral for Australasian and American marsupials. Here we compare the distribution of the (T(2)AG(3))( n ) sequence and constitutive heterochromatin in the presumed ancestral 2n = 14 complement and in complements with known rearrangements. We found that where there were moderate to large amounts of constitutive heterochromatin, the distribution of the (T(2)AG(3))(n) sequence reflected its presence as a native component of satellite DNA rather than its involvement in past rearrangements. The presence of centromeric heterochromatin in all Australian 2n = 14 complements therefore suggests that centromeric sites of the (T(2)AG(3))(n) sequence do not represent evidence for recent rearrangements.