Phenotypic and Functional Characterization of Monoclonal Antibodies with Specificity for Rhesus Macaque CD200, CD200R and Mincle

Lectin-like molecules and their receptors are cell surface molecules that have been shown to play a role in either facilitating infection or serving as transporters of HIV/SIV in vivo. The role of these lectin-like molecules in the pathogenesis of HIV/SIV infection continues to be defined. In efforts to gain further insight on the potential role of these lectin-like molecules, our laboratory generated monoclonal antibodies (mAb) against the human analogs of rhesus macaque CD200, CD200R and Mincle, since the rhesus macaques are accepted as the most reliable animal model to study human HIV infection. The characterization of the cell lineages from the blood and various tissues of rhesus macaques that express these lectin-like molecules are described herein. Among the mononuclear cells, the cells of the myeloid lineage of rhesus macaques are the predominant cell lineages that express readily detectable levels of CD200, CD200R and Mincle that is similar to the expression of Siglec-1 and Siglec-3 reported by our laboratory earlier. Subset analysis revealed that a higher frequency of the CD14⁺/CD16^- subset from normal rhesus macaques express CD200, CD200R and Mincle. Differences in the frequencies and density of expression of these molecules by the gated population of CD14⁺ cells from various tissues are noted with PBMC and bone marrow expressing the highest and the mononuclear cells isolated from the colon and ileum expressing the lowest levels. While a significant frequency of pDCs and mDCs express Siglec-1/Siglec-3, a much lower frequency expresses CD200, CD200R and Mincle in PBMCs from rhesus macaques. The mAb against CD200 and CD200R but not Mincle appear to inhibit the infection of macrophage tropic SIV/SHIV in vitro. We conclude that these mAbs may have potential to be used as adjunctive therapeutic agents to control/inhibit SIV/HIV infection.     

Haemoglobin Polymorphism in the Rhesus Macaque

INTRASPECIFIC polymorphism of the principal haemoglobin component is common among macaque monkeys^1–3 and other non-human primates^4–9, but although electrophoretically demonstrable it has not been found in populations of rhesus monkeys (M. mulatto)^10,11. Using the technique of isoelectric focusing in acrylamide gel, I have found variant haemoglobins in many samples of rhesus red blood cell haemolysates. The detection of these variants is apparently a result of the greatly increased resolution of the isoelectric focusing method as compared with the older electrophoretic methods.     

猴免疫缺陷病毒（SIV）在艾滋病模型恒河猴组织中的分布和载量测定

目的研究当艾滋病恒河猴模型的血浆病毒载量处于低水平或阴性时,猴免疫缺陷病毒（simian immunodeficiency viruses,SIV）在宿主组织中的分布情况。方法SIVmac251感染恒河猴10只,定期检测其血浆载量,感染病毒平均高峰时间第14天时,活检取淋巴结。选取感染18个月后病毒载量最低水平和阴性的2只艾滋病猴（SAIDS）,经安死术后取淋巴结、脾、肝、肺、肾、脑等组织,用原位杂交和实时荧光定量PCR的方法检测病毒在组织中的分布和组织中的病毒载量。结果感染后14d,10只猴血浆病毒载量达到10^7copies/mL,淋巴结组织病毒载量为10^5-10^8copies/g,原位杂交方法在腹股沟淋巴结中检测到强阳性斑点。感染后第18个月的2只猴,血浆病毒载量下降并维持不高于10^2copies/mL水平或阴性,但组织分布不尽相同,在肠系膜淋巴结、肾上腺、海马回、空肠、脾脏等组织中检测到10^5-10^6copies/g的病毒载量,于一只猴的脑积液中检测到10^3copies/mL的病毒载量。用原位杂交的方法在肠系膜淋巴结和空肠中检测到强阳性斑点,其它组织中未检测到阳性斑点。结论实验证实SAIDS猴在血浆病毒载量低甚至阴性时,病毒在不同组织中仍有分布,有些组织中甚至出现高病毒载量,提示在制备SIV/SAIDS模型中,尤其在药物筛选和疫苗评价时,应考虑组织病毒载量指标的测定和药物、疫苗对组织病毒的治疗清除作用的评价。     

中国猕猴遗传多样性研究进展

从形态学、染色体、蛋白质、DNA水平等方面对中国猕猴的遗传多样性进行了综述,以期为我国猕猴资源的保护和利用提供理论基础,为猕猴遗传多样性的研究提供参考.染色体核型和蛋白质分析表明中国猕猴遗传多样性有限,DNA多态性分析表明中国猕猴具有丰富的遗传多样性.基于线粒体控制区部分序列的分析有助于中国猕猴系统发育与进化的研究,Neighbor-joining进化树和Median-Joining网络图将中国猕猴分为7个类群.     

The Rhesus Macaque (Macaca mulatta) Sperm Proteome

Mass spectrometry based proteomics has facilitated sperm composition studies in several mammalian species but no studies have been undertaken in non-human primate species. Here we report the analysis of the 1247 proteins that comprise the Rhesus macaque (Macaca mulatta) sperm proteome (termed the MacSP). Comparative analysis with previously characterized mouse and human sperm proteomes reveals substantial levels of orthology (47% and 40% respectively) and widespread overlap of functional categories based on Gene Ontology analyses. Approximately 10% of macaque sperm genes (113/1247) are significantly under-expressed in the testis as compared with other tissues, which may reflect proteins specifically acquired during epididymal maturation. Phylogenetic and genomic analyses of three MacSP ADAMs (A-Disintegrin and Metalloprotease proteins), ADAM18-, 20- and 21-like, provides empirical support for sperm genes functioning in non-human primate taxa which have been subsequently lost in the lineages leading to humans. The MacSP contains proteasome proteins of the 20S core subunit, the 19S proteasome activator complex and an alternate proteasome activator PA200, raising the possibility that proteasome activity is present in mature sperm. Robust empirical characterization of the Rhesus sperm proteome should greatly expand the possibility for targeted molecular studies of spermatogenesis and fertilization in a commonly used model species for human infertility.The application of mass spectrometry (MS) based proteomics, coupled with whole genome annotation of an increasing number of species, has greatly extended our knowledge of sperm composition. Traditional methods used to assess sperm composition, including the use of sperm-specific antibodies and 2D gel electrophoresis, have identified a limited number of sperm proteins. These traditional studies have been augmented in recent years by the use of high throughput and highly sensitive MS (shotgun proteomics) that have substantially increased the accuracy of peptide identification, resulting in a significant increase in proteome coverage. Indeed, advances in MS instrumentation, data acquisition, and the availability of genome annotations have, for example, increased sperm proteome coverage in Drosophila from 381 (1) to 1108 proteins (2) over a five year period.Two main MS based methodologies have been applied to study sperm composition, including (i) 2D PAGE followed by spot excision and MS and (ii) digestion of proteins, followed by MS/MS analysis of the resulting peptides (3). Although each method has its own advantages and disadvantages, a far greater level of proteome coverage is obtained using MS/MS (4). A previous comparative study found that each method identified proteins not found in the other and vice versa, and therefore it has been suggested that these methods should be used to complement each other (5). Thus, although no single methodology yet exists capable of producing a complete whole cell proteome, MS/MS methods provide deeper and broader coverage and are therefore the current method of choice. Shotgun proteomics has characterized sperm proteomes in a variety of taxa including plants, invertebrates and mammals such as human, mouse, rat, and bull (3, 6–11). These studies achieve varying levels of proteome coverage as a result of several factors including the choice of MS equipment, sample acquisition, purification, solublization, and fractionation schemes. Although these different approaches make direct comparisons difficult they nevertheless have provided invaluable information regarding the composition of sperm and have helped to identify novel proteins that play important roles in sperm function and reproduction.In this study we use MS based proteomics to elucidate the sperm proteome of a species of old world monkey, the Rhesus macaque (Macaca mulatta). Due primarily to their genetic and physiological similarities to humans, Rhesus macaques are the most widely used nonhuman primate model system for basic and applied biomedical research (12). Rhesus macaques are also used extensively as a model of human reproduction where numerous similarities at the molecular level have been observed between gametes of the two species, and why Rhesus macaques have become a useful model system for fertility and assisted reproductive technology research (13). A more complete knowledge of the sperm proteome will facilitate reproductive studies using the Rhesus macaque as a model organism. However, despite its widespread use in reproductive biology, the macaque sperm proteome (MacSP)¹ has yet to be characterized.Although insight into the MacSP will facilitate reproductive studies using the Rhesus macaque as a model organism, this knowledge can also be used to better understand the composition of human sperm. Sperm mature and gain fertilization competency as they traverse the epididymis, a specialized duct that connects the testis to the vas deferens (14). During the maturation process, sperm lose or modify a number of their surface proteins and gain additional transient or permanent surface proteins in a well-organized manner, and it is only after emerging from the cauda epididymis that sperm are motile and considered fertilization competent (14, 15).Proteomic studies of human sperm have been undertaken (3, 6, 10), identifying between 98–1760 sperm proteins, however these studies used sperm from ejaculates which complicates sperm proteome analysis. A previous study identified 923 proteins present in human seminal plasma (16), which is likely to be only a fraction of the seminal plasma proteome. Human sperm proteome data sets derived from human ejaculates makes it difficult to differentiate which of the identified proteins are sperm or seminal plasma constituents. For example, a major seminal protein family, the semenogelins are not expressed in the testis but are found in sperm proteomes determined from ejaculates (6, 10). Such highly abundant seminal proteins may mask lower abundance integral sperm proteins and inhibit their identification by MS. In order to avoid these problems, we collected mature sperm directly from the cauda epididymis of the Rhesus macaque, thus avoiding contamination from seminal plasma proteins.In the present study, sperm proteins were separated using 1D SDS-PAGE, digested and the resulting peptides analyzed by LC MS/MS. Using high stringency parameters for peptide identification, we conservatively identified 1247 proteins from purified samples of Rhesus macaque sperm. Given their close evolutionary relationship, the Rhesus macaque and human share 93% nucleotide homology (12). Data from this study can be used to complement what is currently known about the composition of human sperm and provides a more useful proxy of human sperm proteome composition than the proteomes of other non-primate mammals for which data is available. Studies of sperm composition, especially those in human, can be applied to develop novel molecular based clinical diagnostic tests of sperm quality, which is currently limited to evaluating parameters such as sperm count, morphology and motility. In addition, knowledge of sperm components can lead to the discovery of novel contraceptives and infertility treatments.     

Changes In Rhesus Macaque 'Coo' Vocalizations during Early Development

In order to test whether ‘coo’ calls of young rhesus macaques, Macaca mulatta, undergo some modifications during early development, and to explore which factors may influence these changes, we studied the ontogeny of their contact call, the ‘coo’ call. Vocalizations were recorded during brief periods of social separation. Infants were either raised with their mothers and other conspecifics, or separated from their mothers at birth and housed in a nursery with other infants. We recorded calls uttered in the separation context from 20 infants. We digitized the first 50 calls of a given series and subjected them to a Fourier transform. From each frequency–time spectrum, we extracted 65 acoustic parameters using a software program (LMA 5.9). We then used a cluster analysis to separate the ‘coo’ calls from other call types. With increasing age, the ‘coos’ dropped in pitch and became more even. The course of amplitude became more constant and the call duration increased slightly. Nevertheless, we found a high intra‐individual variation throughout the 5 mo. Neither rearing condition nor sex had any apparent influence on age‐related changes in ‘coo’ structure. With one exception, all parameters that correlated with age could be explained by variation in weight. Therefore, we conclude that growth is the main factor accounting for the observed changes.     

喀斯特生境中猕猴的活动节律和时间分配

2006年9月至2007年8月,在广西弄岗国家级自然保护区选择一群猕猴(Macaca mulatta)作为观察对象,采用瞬时扫描取样法收集相关的行为数据,以日活动节律和活动时间分配为切人点,探讨猕猴对喀斯特石山生境的行为适应策略.结果表明,猕猴的日活动节律表现为上午和下午的觅食高峰,中午进入长时间的休息期.这可能与白天...     

Mineralized Trichobezoars in a Rhesus Macaque (Macaca mulatta)

A five-year-old female rhesus macaque (Macaca mulatta) presented with a thin body condition and multiple palpable mid-abdominal masses. Mineralized cecal trichobezoars were removed surgically. Thirteen months later, similar masses recurred and were confirmed with radiographs. This is the first case report of a mineralized cecal trichobezoar in a rhesus macaque.     

Identification of the Rhesus Macaque Rhadinovirus Lytic Origin of DNA Replication

We have identified a lytic origin of DNA replication (oriLyt) for rhesus macaque rhadinovirus (RRV), the rhesus macaque homolog of human herpesvirus 8 (HHV-8), also known as Kaposi's sarcoma-associated herpesvirus. RRV oriLyt maps to the region of the genome between open reading frame 69 (ORF69) and ORF71 (vFLIP) and is composed of an upstream A+T-rich region followed by a short (300-bp) downstream G+C-rich DNA sequence. A set of overlapping cosmids corresponding to the entire genome of RRV was capable of complementing oriLyt-dependent DNA replication only when additional ORF50 was supplied as an expression plasmid in the transfection mixture, suggesting that the level of ORF50 protein originating from input cosmid DNA was insufficient. The requirement of RRV ORF50 in the cotransfection replication assay may also suggest a direct role for this protein in DNA replication. RRV oriLyt shares a high degree of nucleotide sequence and G+C base distribution with the corresponding loci in HHV-8.     

恒河猴基因组SINEs和Alu元件的数量和分布

哺乳动物的基因组中富含各种类型的重复序列,其中的微卫星作为分子标记在相关研究中得到了广泛的应用。而重复序列中的SINEs元件,在各类群物种的分子系统发育、遗传多样性等方面的研究也得到了使用。其中,灵长类物种特有的SINEs元件、Alu元件,也在灵长类物种的进化研究中得到了成功的使用。本研究对于重要的医学模式动物恒河猴的基因组中SINEs和Alu元件进行了搜索,并进一步统计分析其分布规律、长度等信息。在恒河猴基因组的20条常染色体上共发现了Alu元件1 093 185个,在性染色体X上发现了45 215个。长度为200 bp至300 bp区间的Alu元件分布最多;Alu元件中75%的分化值至少都为10,而只有6.2%左右的元件分化值能达到至少20,这一结果表明绝大部分的Alu元件都比较年轻。本研究的统计结果为后续应用SINEs和Alu元件作为分子标记的研究提供了重要的信息。     

The Peculiar Evolution of Apolipoprotein(a) in Human and Rhesus Macaque

Apo(a) is a low density lipoprotein homologous to plasminogen and has been shown to be involved in coronary atheroschlerosis. In the present paper we will try to analyze the interesting evolutionary pattern of Apo(a). The plasminogen gene contains 5 cysteine-rich sequences, called kringles, followed by a protease domain. Apo(a), probably arisen by duplication of an ancestral plasminogen gene, contains many tandemly repeated copies of a sequence domain similar to the fourth kringle of plasminogen, 37 in human and at least 10 in the partially sequenced gene of rhesus, and the protease domain. We have found that the upstream kringles of apo(a) undergo Molecular Drive-like processes that produce high intraspecies similarity, whereas the downstream kringles evolve in a molecular clock-like manner and show an high interspecies sequence similarity. The latter regions are obviously suitable for dating the duplication event by which Apo(a) arose from plasminogen, but only if they evolve at the same rate in the two genes. Thus, we propose a ``Molecular Clock Test' for assessing whether the comparison of two paralogous genes (or gene regions) can give reliable information on the dating of their origin by duplication. Applying this test to the kringle-4 domain of apo(a) and plasminogen gene, we demonstrate that the separation between the two genes by duplication dates back at about 90 Mya immediately before the radiation of mammals.     

Multi-dose Romidepsin Reactivates Replication Competent SIV in Post-antiretroviral Rhesus Macaque Controllers

Viruses that persist despite seemingly effective antiretroviral treatment (ART) and can reinitiate infection if treatment is stopped preclude definitive treatment of HIV-1 infected individuals, requiring lifelong ART. Among strategies proposed for targeting these viral reservoirs, the premise of the “shock and kill” strategy is to induce expression of latent proviruses [for example with histone deacetylase inhibitors (HDACis)] resulting in elimination of the affected cells through viral cytolysis or immune clearance mechanisms. Yet, ex vivo studies reported that HDACis have variable efficacy for reactivating latent proviruses, and hinder immune functions. We developed a nonhuman primate model of post-treatment control of SIV through early and prolonged administration of ART and performed in vivo reactivation experiments in controller RMs, evaluating the ability of the HDACi romidepsin (RMD) to reactivate SIV and the impact of RMD treatment on SIV-specific T cell responses. Ten RMs were IV-infected with a SIVsmmFTq transmitted-founder infectious molecular clone. Four RMs received conventional ART for >9 months, starting from 65 days post-infection. SIVsmmFTq plasma viremia was robustly controlled to <10 SIV RNA copies/mL with ART, without viral blips. At ART cessation, initial rebound viremia to ~10⁶ copies/mL was followed by a decline to < 10 copies/mL, suggesting effective immune control. Three post-treatment controller RMs received three doses of RMD every 35–50 days, followed by in vivo experimental depletion of CD8⁺ cells using monoclonal antibody M-T807R1. RMD was well-tolerated and resulted in a rapid and massive surge in T cell activation, as well as significant virus rebounds (~10⁴ copies/ml) peaking at 5–12 days post-treatment. CD8⁺ cell depletion resulted in a more robust viral rebound (10⁷ copies/ml) that was controlled upon CD8⁺ T cell recovery. Our results show that RMD can reactivate SIV in vivo in the setting of post-ART viral control. Comparison of the patterns of virus rebound after RMD administration and CD8⁺ cell depletion suggested that RMD impact on T cells is only transient and does not irreversibly alter the ability of SIV-specific T cells to control the reactivated virus.     

SHIV-KB9感染中国恒河猴动物模型的建立

目的为了进一步确证SHIV-KB9感染中国恒河猴的病毒浓度范围,测试动物对病毒的适应性,明确该动物模型的可重复性。方法实验前采集猴血清并进行血清学检查。选出4只无SIV、STLV、SRV/D和B病毒感染的恒河猴,分别用10倍系列稀释的病毒液静脉感染实验猴,使用流氏细胞术、血常规、病毒分离、DNA-PCR和RT-PCR等方法确定实验猴是否被感染,以及感染后恒河猴体内病毒复制和免疫细胞损伤情况。结果实验猴的血浆病毒载量、病毒分离结果、CD4＋/CD8＋比值和CD4＋T细胞数等证实,4.8×105 copies/mL以上浓度的SHIV-KB9病毒液能成功感染中国恒河猴。结论本研究进一步明确了SHIV-KB9感染中国恒河猴的有效病毒浓度范围,确定了SHIV-KB9病毒感染中国恒河猴的病毒学、免疫学的测定指标,成功的建立了SHIV-KB9/中国恒河猴动物模型。     

圈养猕猴志贺氏菌的分离鉴定及药敏分析

目的确定猕猴感染志贺氏菌的状况,寻找有效治疗措施。方法采用不同选择培养基对13份病猴粪便样品进行分离培养、细菌革兰氏染色、镜检,并对分离的疑似菌株进行细菌生化鉴定和分子鉴定,经小白鼠致病性实验后,再用纸片扩散法测定分离菌株对23种抗生素的敏感性。结果从13份猕猴粪便样品中共检出12株志贺氏菌,检出率为92.31%,其中痢疾志贺菌(A群)1株、福氏志贺菌(B群)10株、宋内氏志贺菌(D群)1株;致病性试验结果表明,12株菌均能在72h内致死小白鼠,并能回收到注射的菌株;药敏试验结果表明,本实验中分离到的志贺氏菌对头孢噻肟(86.49%)最敏感,对头孢三嗪(75.00%)、头孢他啶(66.67%)次之,对多粘菌素B、羧苄西林、苄唑西林素等抗生素耐药性强。结论初步确定猕猴感染志贺氏菌普遍存在,进而引起腹泻、痢疾的可能性较大,头孢噻肟等为最敏感药物。